Consequences of Eukaryotic Enhancer Architecture for Gene Expression Dynamics, Development, and Fitness
The regulatory logic of time- and tissue-specific gene expression has mostly been dissected in the context of the smallest DNA fragments that, when isolated, recapitulate native expression in reporter assays. It is not known if the genomic sequences surrounding such fragments, often evolutionarily conserved, have any biological function or not. Using an enhancer of the even-skipped gene of Drosophila as a model, we investigate the functional significance of the genomic sequences surrounding empirically identified enhancers. A 480 bp long “minimal stripe element” is able to drive even-skipped expression in the second of seven stripes but is embedded in a larger region of 800 bp containing evolutionarily conserved binding sites for required transcription factors. To assess the overall fitness contribution made by these binding sites in the native genomic context, we employed a gene-replacement strategy in which whole-locus transgenes, capable of rescuing even-skipped- lethality to adulthood, were substituted for the native gene. The molecular phenotypes were characterized by tagging Even-skipped with a fluorescent protein and monitoring gene expression dynamics in living embryos. We used recombineering to excise the sequences surrounding the minimal enhancer and site-specific transgenesis to create co-isogenic strains differing only in their stripe 2 sequences. Remarkably, the flanking sequences were dispensable for viability, proving the sufficiency of the minimal element for biological function under normal conditions. These sequences are required for robustness to genetic and environmental perturbation instead. The mutant enhancers had measurable sex- and dose-dependent effects on viability. At the molecular level, the mutants showed a destabilization of stripe placement and improper activation of downstream genes. Finally, we demonstrate through live measurements that the peripheral sequences are required for temperature compensation. These results imply that seemingly redundant regulatory sequences beyond the minimal enhancer are necessary for robust gene expression and that “robustness” itself must be an evolved characteristic of the wild-type enhancer.
Published in the journal:
. PLoS Genet 7(11): e32767. doi:10.1371/journal.pgen.1002364
Category:
Research Article
doi:
https://doi.org/10.1371/journal.pgen.1002364
Summary
The regulatory logic of time- and tissue-specific gene expression has mostly been dissected in the context of the smallest DNA fragments that, when isolated, recapitulate native expression in reporter assays. It is not known if the genomic sequences surrounding such fragments, often evolutionarily conserved, have any biological function or not. Using an enhancer of the even-skipped gene of Drosophila as a model, we investigate the functional significance of the genomic sequences surrounding empirically identified enhancers. A 480 bp long “minimal stripe element” is able to drive even-skipped expression in the second of seven stripes but is embedded in a larger region of 800 bp containing evolutionarily conserved binding sites for required transcription factors. To assess the overall fitness contribution made by these binding sites in the native genomic context, we employed a gene-replacement strategy in which whole-locus transgenes, capable of rescuing even-skipped- lethality to adulthood, were substituted for the native gene. The molecular phenotypes were characterized by tagging Even-skipped with a fluorescent protein and monitoring gene expression dynamics in living embryos. We used recombineering to excise the sequences surrounding the minimal enhancer and site-specific transgenesis to create co-isogenic strains differing only in their stripe 2 sequences. Remarkably, the flanking sequences were dispensable for viability, proving the sufficiency of the minimal element for biological function under normal conditions. These sequences are required for robustness to genetic and environmental perturbation instead. The mutant enhancers had measurable sex- and dose-dependent effects on viability. At the molecular level, the mutants showed a destabilization of stripe placement and improper activation of downstream genes. Finally, we demonstrate through live measurements that the peripheral sequences are required for temperature compensation. These results imply that seemingly redundant regulatory sequences beyond the minimal enhancer are necessary for robust gene expression and that “robustness” itself must be an evolved characteristic of the wild-type enhancer.
Introduction
The genetic code, a simple one-dimensional vector of only four symbols, is decoded for the most part by molecular machinery that adheres to a strict grammar for translating genetic information into functional molecules. The specificity of the genetic code forms the conceptual basis for constructing “annotated” genomes, a major effort of the post-genome sequencing era.
But the majority of functional information in a genome does not reside in its transcribed compartments, where this strict grammar applies, but rather in the vast sea of “noncoding” sequences specifying the regulatory logic of gene expression. For these sequences, and in particular for the cis-regulatory elements (CRE) controlling eukaryotic gene expression, originally called enhancers [1], there is as yet no general agreement about how to define, much less identify the “functional” unit of eukaryotic gene regulation [2], [3], [4], [5], [6]. Enhancers generally contain multiple closely spaced target binding sites for several distinct transcription factors [7], [8], an attribute that can be exploited to identify enhancer sequences in silico [5], [9], [10], [11], [12], [13]. The best definition of a CRE, however, remains a time-tested functional one – the smallest piece of contiguous DNA that is capable of recapitulating a spatio-temporal pattern of native gene expression when placed in front of a promoter and reporter gene (typically β-galactosidase or GFP) and reintroduced into the organism from which the sequence was taken [7]. We will refer to these experimentally defined CRE's as “minimal” elements or enhancers.
Experimentally defined enhancers have discrete physical boundaries necessarily, but such discreteness is difficult to justify biologically. Sequences to which a transcription factor (TF) binds can only be described probabilistically [14], [15], owing to the fact that binding is not to unique target but rather to variants of a short sequence motif. TF binding occurs, therefore, not only at canonical or “high affinity” sites —ones that are typically identified in in vitro assays— but also to numerically abundant “low affinity” sequences [16], which are ever-present both within and beyond the margins of minimal enhancers. Evidence for their functionality comes primarily from modeling gene expression: weaker bioinformatically-identified sites are required to correctly predict activity [17], some taking the extreme approach of including all possible TF-DNA occupancy configurations [18], [19].
Furthermore, it is also not always possible to decompose the sequences contributing to activity in a tissue into discrete units. The expression in stripe 7 of the Drosophila melanogaster even-skipped (eve) gene receives contributions both from sequences in the “3+7” enhancer and from proximal sequences [17], [20], [21]. Similarly, the dorsal expression of shavenbaby in larval trichomes is derived from both the “E” and “7” enhancers [22] and both anterior and posterior giant (gt) domains receive input from multiple enhancers [23].
A lack of discrete CRE boundaries is also evident in the evolutionary analysis of binding site gain and loss, commonly referred to as “binding site turnover”. Comparing CRE sequences between the sibling species' D. melanogaster and D. simulans reveals the loss or gain of approximately 5% of transcription factor binding sites (TFBS) that have been functionally validated in well-characterized D. melanogaster enhancers [24], [25]. Binding site loss in D. simulans is expected to be offset by the gain of novel sites for the same TF, but this is not the case if the search for predicted new sites is restricted to the intervals identified as CREs in D. melanogaster. Additional novel binding sites are identifiable, however, if the search interval is expanded by 200bp in either direction, thus implying a functional role for these flanking sequences.
It is also not uncommon to find evolutionarily conserved instances of a TFBS beyond the borders of a minimal CRE, as exemplified by the Drosophila eve stripe 2 enhancer (S2E) [26], [27], the subject of this investigation. The eve minimal stripe 2 element (MSE), arguably the most intensively studied of all eukaryotic enhancers, constitutes a 480bp noncoding fragment located approximately 1000bp upstream of transcription initiation [20], [28] and contains a total of 12 “strong” TF binding sites, six sites for the activators Bicoid (Bcd) and Hunchback (Hb) and six sites for the repressors Krüppel (Kr) and Gt, as well as several additional “weak” Kr sites [29], [30]. In vitro DNAase footprinting experiments also identified three additional Kr binding sites beyond the borders of the minimal enhancer as well as two additional Hb sites [29]. But these binding sites appear to be redundant for S2E expression since the minimal element lacking them can direct a transverse band of expression in the blastoderm embryo at the same location as the native eve stripe 2 [31], [32], [33]. Comparative analysis of sequences across Drosophila phylogeny, however, indicates that all but possibly one site (hb-1) are conserved to the same extent as many sites internal to the MSE, indicating that they are functional [27].
The empirical definition of the enhancer itself, with discreteness as its conceptual underpinning, has yet to be put to experimental test. Accordingly, we ask here whether the MSE recovers the complete biological activity of the wildtype enhancer, that is, whether the conserved flanking binding sites are redundant or not.
Among the many biological characteristics of enhancer activity we could measure, we wished to investigate possible differences in the functional robustness of the MSE versus wildtype S2E for the following reason: an enhancer is expected to evolve not simply as a regulatory switch to turn gene expression on or off in response to a set of upstream signals, but also to do so “correctly” across the range of variability found in the signaling system. This variability is expected to arise by intrinsic molecular noise [34], [35], [36], [37], [38], [39], [40], [41], genetic variability in upstream factors and processes [42], [43], [44], as well as by external environmentally imposed conditions, such as the temperature-dependent rate of development [34], [45]. We hypothesize that certain features of enhancer architecture, such as the multiplicity of binding sites for a transcription factor, have evolved to assure stable enhancer performance rather than its switch-like behavior per se. Under this hypothesis, novel binding sites that make the enhancer more “robust” to perturbation will be selectively favored and will thus be incorporated into the enhancer architecture by a process of accretion [46]. The periphery of a CRE, we further hypothesized, might be a good place to look for the presence of such functional elements. Comparing the performance of the eve MSE versus the wildtype S2E would allow us to test this hypothesis.
To answer these questions we employed several experimental innovations. First, we investigated the temporal dynamics of stripe formation in individual live embryos, a characteristic of developmental robustness not observable with fixed, stained embryos. For this purpose, we created a fusion of the Eve protein with the fluorescent protein SYFP2, a fast-folding variant of the Yellow Fluorescent Protein (henceforth called YFP), to allow temporally resolved measurements of Eve stripe formation. A “live Eve” system also allowed us to synchronize the measurements across embryos to a specific nuclear division so that we could observe events in “wall-clock” time, independent of the status of developmental markers of pattern formation. The fusion protein additionally allowed us to measure not only Eve stripe 2 driven by either the MSE or the wildtype enhancer but all seven Eve stripes simultaneously. The additional stripe information internal to each embryo, genetically invariant landmarks surrounding stripe 2, allowed us not only to better characterize stripe 2 phenotypes, but also to investigate novel aspects of stripe formation dynamics. We could also investigate the robustness of enhancer performance in embryos developing at different growth temperatures.
Second, advances in transgene construction technology made it possible to investigate the S2E in a ∼16.4 kb transgene containing the entire native eve locus [26], [47]. Specifically, we investigated the eve locus (1) with the complete and unaltered S2E in its native context; (2) with the two regions flanking the MSE that contain the additional mapped Kr and Hb sites deleted, leaving behind the MSE sequence to drive eve stripe 2 expression; and (3) with an inverted version of the MSE to test the importance of enhancer orientation.
Third, we used site-directed transgenesis to place each version of the eve locus into the same target site in the Drosophila genome [48], [49]. All comparisons, therefore, were carried out in co-isogenic strains, eliminating any potential position effect of transgene insertion. Finally, genetic crosses allowed us to eliminate the functional native eve locus and to replace it with the whole-locus transgene copy. In doing so, we could investigate developmental phenotypes such as engrailed (en) expression, or fitness traits such as viability, in addition to molecular aspects of stripe formation. The ability to examine molecular, developmental, and organismal phenotypes with this novel experimental system allowed us to establish the molecular causality of defects occurring later in the life cycle of the fly, and therefore to establish a more complete biology of the MSE versus wildtype eve stripe 2 regulatory element.
Results
Our strategy was to create co-isogenic lines differing only in the S2E sequence carried by the transgenic eve locus. Three versions of the eve-YFP transgene were constructed: WT, which contains the “wildtype” reference stripe 2 enhancer sequence; MSE, which has a truncated stripe 2 enhancer; and INV_MSE, which has the orientation of the truncated stripe 2 enhancer inverted (Figure 1). Co-isogenic strains were created by targeting transgene insertion to the attP2 docking site. As we will show in the following section, a wildtype eve locus transgene lacking the YFP fusion, targeted to the attP2 site, delivers nearly full adult viability when it replaces the native eve locus.
The results are presented in three sections. The first section addresses a fundamental biological question: Do the MSE and INV_MSE versions of the transgene make a viable fly (e.g., are they less fit than WT)? To measure eve transgene viability, we eliminated the native eve locus by crossing the transgene into one of three eve mutant backgrounds: eveR13 (R13), a null allele created by a coding point mutation; Df(2R)eve (Df(eve)), a small deletion covering the entire eve locus and its immediate neighbors, and eveΔMSE, the native locus in which the MSE region of the stripe 2 enhancer is deleted and replaced with w+ sequence (Figure 1A). The recovery of complete wildtype viability when only transgenic eve is available is a stringent test of the suitability of the target site and whole-locus transgene for the proposed experiments. Next we compare the viability of WT, which encodes the Eve-YFP fusion, to that of the unmodified eve transgene to test the YFP tag's effect on the panoply of eve function. The recovery of good viability in WT permitted us to investigate the extent to which adult viability is compromised when eve stripe 2 expression is driven by either MSE or INV_MSE.
Section two reports the effects of WT, MSE, and INV_MSE on Engrailed patterning in an attempt to link differences in the viability in the two MSE genotypes compared to WT to Eve stripe-2-specific segmentation defects.
Having established this link, we present in the third section a detailed analysis and comparison of in vivo eve stripe 2 expression phenotypes. We first present experimental results that compare Eve-YFP and Eve expression to establish the fidelity of the Eve-YFP reporter. This is followed by a detailed analysis of Eve stripe 2 initiation, maturation and precision of border placement in WT, MSE, and INV_MSE. The section closes with an analysis of the response of stripe 2 expression phenotypes to embryonic growth temperature.
Viability
To avoid complications of position effect on gene expression, all the studied transgenes were integrated into the same chromosome 3 attP2 docking site (3L [68A4]) [49]. To establish the suitability of this target site for expressing eve, we created a fly line, attP2[S2EwtEVEwt] (henceforth called EVE), in which the 16.4 kb unmodified native eve locus, sans a YFP tag or any modification to the S2E, was integrated into the target site. We evaluated the ability of this transgene to restore egg-adult viability when crossed into an Eve null (R13) genetic background (Figure 2A; Table S1).
The wildtype eve transgene (EVE) yielded very high homozygous rescue percentages (80 – 85%)—more than twice the corresponding rescue percentages previously reported for a slightly smaller version of the transgene [26], [47], [50] (also Methods)— that were not significantly different from full 100% rescue (p>0.5; Figure 2B; Table S1). Unless otherwise stated, all statistical testing for viability used the chi-squared test. The improvement in rescue ability may be due either to properties of the attP2 target site and/or to the inclusion of an additional sequence at the 3′ end of the transgene that contains insulator binding sites (Methods). Hemizygous rescue percentages are lower than for homozygotes, as expected for this haplo-insufficient locus [50], [51]. No significant difference was observed in the recovery of males versus females for either the hemizygous (p = 0.43) or homozygous (p = 0.88) rescue classes, a point to which we return in the following section.
Impact of YFP tag on fly viability
To monitor Eve stripe formation, we constructed the real-time 4D reporter eve transgene, WT (attP2[S2EwtEVEYFP]), by fusing a YFP-encoding sequence to the C-terminal of the eve coding region (Figure 1B). We first investigated the impact of the YFP tag in WT on egg-adult viability, a sensitive biological indicator of the fusion protein's effect on Eve protein function. The estimated rescue percentages of WT were consistently lower than for the corresponding eve transgene lacking the YFP tag (Figure 2B, Tables S1 and S2), but a robust proportion of adults of both homozygous and hemizygous genotypes were recovered. Therefore, although the YFP tag does reduce lifetime fitness, its overall functional impact is modest.
Minimal stripe enhancers make a viable fly
Having established the functionality of the fusion transgene (WT), we proceeded to investigate the impact of removing sequences in the stripe 2 enhancer region to create two “minimal” stripe 2 enhancers, MSE (attP2[S2EMSEEVEYFP]) and INV_MSE (attP2[S2EINV_MSEEVEYFP]). Can the eve locus with a total of 244bp of DNA deleted from the stripe 2 enhancer region, eliminating two footprinted binding sites each for the transcription factors Kr and Hb (kr-2, kr-1, hb-2 and hb-1), make a sufficiently functional stripe to produce a viable fly?
To our surprise, flies homozygous for either MSE or INV_MSE in an R13 (native eve null) background were both highly viable (Figure 2B) and fertile (data not shown). MSE relative viability was not significantly reduced compared to WT for either sex (p(males) = 0.28; p(females) = 0.36). INV_MSE homozygotes also did not exhibit reduced survival, and in fact showed significantly higher survival than WT (p(males) < 0.005; p(females) = 0.01).
Two conclusions can be drawn from these observations. First, the fact that the MSE transgene, the smallest DNA fragment capable of recapitulating a stripe 2 in a reporter assay, is sufficient to produce a biologically functional Eve stripe, provides a strong validation of the empirical reporter approach to identifying functional units of cis-regulatory DNA. Moreover, the fact that INV_MSE is also biologically active confirms the S2E's conformity to orientation independent functionality, a fundamental principle of enhancer activity [1]. Second, physically mapped and evolutionarily conserved transcription factor binding sites for Kr and Hb that are deleted in MSE are not required for the enhancer to function biologically. Sequence conservation, in this context, does not equate to functional essentiality.
Although MSE and INV_MSE restores full viability when homozygous, it might be argued that this viability is not so much a function of the minimal enhancers delivering wildtype activity but rather the ability of the developmental system to buffer against variation in Eve stripe 2 expression. To test this hypothesis, we investigated the ability of MSE and INV_MSE to restore viability under more challenging conditions — when only one copy of the transgene was present in a fly. Strongly supporting the hypothesis, hemizygous MSE or INV_MSE exhibited strongly reduced adult viability, averaging less than 5%, as compared to ∼30% for WT (Figure 2B, Table S2). This relative reduction in viability must be attributable to functional differences between the MSE and WT versions of the S2E.
Sex ratio
The viability experiments allowed us to compare males and females of a given genotype, and we observed a distortion of the sex ratio favoring females in all genotypic classes and all transgenes (Figure 2B and Table S2), including genotypes carrying a copy of the native eve locus. Of particular interest, however, is a greater relative loss of male viability in MSE homozygotes as compared to WT (p = 0.01), suggesting the possibility of a functional difference in MSE-driven stripe formation between males and females. A similar, and even more severe, trend was seen for the small number of MSE hemizygote survivors compared to WT.
To further investigate this surprising sex-dependent viability loss, we carried out a cross (Figure S1) that is expected to yield 50% hemizygotes (compared to 1/9th in the standard viability assay; see Figure 2A). We again observed a reduction in the viability of hemizygous MSE and INV_MSE compared to WT, but more importantly a 4-6-fold reduction in the recovery of males compared to females (Figure S1, p = 2.3E-23 and p = 1.3E-11, respectively). Two additional crosses further confirmed the sex-dependent viability difference in MSE genotypes. In these crosses the native eve locus was eliminated not with the R13 eve null allele, but with either Df(eve) or eveΔMSE (Figure 1 and Methods). In both crosses, the number of hemizygous males relative to females was reduced in MSE and INV_MSE compared to WT (Figures S2 and S3). The cross with eveΔMSE (Figure S3) was particularly informative in this regard. eveΔMSE/R13 offspring were diploid for all eve cis-regulatory regions except for the S2E — for which they were haploid. In this case the rescue by the WT S2E allele showed no sex bias, whereas the MSE and INV_MSE-rescued males had significantly lower viability (Figure S3, p = 2.1E-5 and p = 0.012, respectively). Similarly, R13/CyO offspring, which were diploid for the regions flanking the minimal enhancer in the WT rescue but haploid in the MSE or INV_MSE rescues, also had significantly lower male viability in MSE and INV_MSE compared to WT (p = 2.2E-5 and p = 0.003, respectively). Therefore for this cross, sex-dependent viability can be specifically attributed to the hemizygosity of the stripe 2 enhancer region in MSE and INV_MSE.
Engrailed patterning
As the reduction in viability of the two hemizygous MSE genotypes (relative to WT) is due only to differences in the enhancer, we can make two predictions: (1) there will be developmental defects in the formation of eve stripe 2-dependent segments in MSE hemizygotes, and (2) these segmentation defects will create lethality at the embryonic stage. To test the latter prediction, we investigated embryo hatching rates from a cross expected to yield 50% hemizygotes in the rescue of R13 by the transgenes (Figure S4). The balancer chromosome was marked with Deformed-YFP (Dfd-YFP) and we measured relative viability by counting Dfd-YFP positive and negative hatched first instar larvae. Under the assumption that the heterozygous genotype w; b,R13/CyO,p[Dfd-YFP]; attP2[S2EA1EVEYFP] has the same relative viability for all three versions the eve transgene (supporting evidence in Methods), prediction (2) can be tested by comparing the proportions of hemizygous WT versus MSE (or INV_MSE) transgene survivors (homozygous for R13). Consistent with this prediction, WT exhibited significantly better viability at this stage of development then either MSE or INV_MSE.
By confirming viability loss at the embryonic stage in MSE and INV_MSE hemizygotes, we proceeded to investigate whether specific defects in segmentation could be observed between the WT, MSE, and INV_MSE. The establishment of the en 14-stripe segment polarity gene expression pattern is a complex process that includes activation by eve early stripes [50]. Eve stripe 2 corresponds to parasegment 3, which is bordered by en stripes 3 and 4. These En stripes are developmental indicators of Eve stripe 2 expression: homozygous eveΔMSE embryos lacking a functional stripe 2 enhancer produce a short parasegment three due to an anterior-shifted and vestigial En stripe 4 (Figure 3A). As expected, eveΔMSE is a recessive embryonic lethal (Figure S5).
We focused attention on the position of En stripe 4 in stage 10 and 11 embryos by measuring its location relative to bordering stripes 3 and 5 (see Methods) in hemizygous embryos (Figure 3B, 3C). Both MSE genotypes exhibited a statistically significant reduction of parasegment 3 (p<0.01) when measured in embryos in which the native eve locus was removed (Df(eve)/R13) (Figure 3D; Table S3). We also investigated the same genotypes in stage 11 embryos when only the stripe 2 enhancer was deleted from the native eve locus (eveΔMSE /R13) and again found a significant reduction of parasegment 3 in MSE (p<0.01, the Mann-Whitney Wilcoxon ranksum test was used here and in all subsequent statistical testing) and nearly significant (p = 0.08) in INV_MSE hemizygotes (Figure S7; Table S4). The segmental defect revealed by En patterning in hemizygous embryos, therefore, can be attributed specifically to hemizygosity of MSE or INV_MSE.
Dynamics of eve stripe 2 expression
The studies of adult viability and En patterning in MSE versus WT, as presented above, establish biological differences that are directly attributable to the structural differences in the enhancer itself. In the following sections, we investigate the dynamics of Eve stripe 2 formation and maturation, taking advantage of the ability to track its evolution in an individual embryo through time.
Differences in En patterning in WT and MSE could be the result of average differences in Eve stripe 2 patterning or greater variation among individual embryos. Analysis of stripe patterning in live embryos allowed us to investigate both features of stripe dynamics. Because the measurements of stripe formation and maturation involves data collected from live embryos, a brief overview of the methods employed and their validation is presented.
Validation of Eve-YFP expression in fixed tissue
In order for eve-YFP to be useful as a live reporter, it must express Eve-YFP protein with a high fidelity to the endogenous Eve pattern in space and time. In an approach similar to the one taken for validating bcd-GFP expression [52], we tested the fidelity of the Eve-YFP pattern at nuclear resolution by co-staining embryos carrying the eve-YFP transgene with anti-Eve and anti-GFP antibodies and measuring the mean fluorescence in each nucleus (see Methods). As shown in Figure S8A, fluorescence in the two channels exhibits a strongly linear relationship. Eve provides positional information in the embryo, and the correct positioning of its borders is essential for normal segmentation [53]. Due to their functional importance, we measured the border positions and found that Eve-YFP forms its borders in the same positions as endogenous Eve (Figure S8D).
Despite strongly proportional expression and identical border positions, closer inspection of overlays of anti-GFP and anti-Eve profiles from the same embryo shows that the Eve-YFP pattern exhibits a temporal lag compared to endogenous Eve (Figure S8B). The lag is less than 6 min since the expression profiles score in the same time class of the staging scheme of Surkova et al. [36]. This delay is perhaps not surprising since the fusion gene is longer than eve and would take more time to be transcribed and translated. The Eve-YFP pattern in fixed tissue shows the same WT, MSE and INV_MSE phenotypes as the live data (Figure S9).
Imaging of Eve-YFP expression in vivo
Since gene expression movies are acquired from each embryo in a separate experiment, we adopted an experimental methodology to ensure that data from individual embryos were comparable (see Methods). One of the strengths of live imaging is the ability to follow gene expression in absolute time without relying on the pattern of Eve maturation or embryo morphology to determine the age of an embryo. Instead, we registered the time series of embryos imaged in separate experiments by starting the clock at the completion of the thirteenth nuclear division, made possible by the presence of a His2Av-RFP transgene to mark nuclei, and were able to determine the age of each embryo relative to the starting point with a precision of 0.5 min (see Methods).
Quantitative Eve-YFP data from live embryos
We used image segmentation techniques to automatically identify nuclei in the His2Av-RFP images and calculated the mean fluorescence intensity of Eve-YFP expression in the pixels lying inside each nucleus (Figure 4, see Methods). Eve-YFP profiles from individual embryos follow the same overall temporal progression as the one observed in fixed tissue (Video S1, [36], [54]. Despite general agreement with the chronology of Eve pattern maturation, the in vivo Eve-YFP pattern appears to lag behind that of endogenous Eve. Using the staging scheme of Surkova et al. [36], the live Eve-YFP patterns score in a time class occurring 15–20 min before the actual age of the embryo (legend of Figure 4A). This delay is much larger than the one observed between fixed-tissue Eve-YFP and Eve profiles. This is not surprising since fluorescent proteins require additional steps after folding to achieve fluorescence [55]. Because the temporal progression of in vivo Eve-YFP expression follows that of endogenous Eve, the main limitation resulting from this lag is that we cannot observe the most mature Eve expression having equally bright stripes [36] seen in the last quarter of cycle 14.
Phenotypes of Eve stripe maturation and initiation
Several Eve stripe 2 phenotypes could be measured in the live-image data. We extracted Eve-YFP profiles from the dorsal and ventral edge of each embryo by projecting onto the anteroposterior (AP) axis. Both profiles exhibit the same phenotypes (Figure 4B), but we restricted further analysis to ventral profiles only as they display the most mature Eve expression. Eve stripe 2 can be described by six features - expression level at the peak, the heights of the two borders, and the positions of the peak and borders (Figure 5A) - that can be detected using a spline approximation (Figure 5B and Methods).
One of the important added values of the eve-YFP fusion in a whole-locus transgene is that all seven Eve stripes are visible in the developing embryos, whereas only stripe 2 varies genetically. This allows us to scale the properties of stripe 2 relative to those of stripe 1, which serves as a within-embryo control on embryo-to-embryo experimental variation. Accordingly, we define two Eve maturation phenotypes, relative activation and relative repression, as the ratio of peak stripe 2 expression to that of stripe 1 and the ratio of the heights of the anterior and posterior borders respectively. The former is a measure of stripe 2 activation, while the latter is a measure of the repression of the anterior border. We present these measurements at three-minute intervals for a total of 18 minutes, from when stripe 2 is first detectable until gastrulation. Inspection of these temporally resolved data allow us to analyze not only the differences between WT and MSE at comparable developmental stages, but also differences in the temporal dynamics of stripe formation.
In addition to these stripe 2 maturation phenotypes, we also used the in vivo movies to investigate two additional phenotypes relating to the appearance of a nascent stripe.
Eve stripe 2 phenotypes at the late cellular blastoderm stage
We first describe stripe 2 differences at the late blastoderm stage just prior to the initiation of gastrulation. The “mature” Eve stripes produced by MSE and INV_MSE exhibit distinct defects compared to WT (Figure 4 and Figure 5C, 5D). The defects involve peak and border heights but not border positions, which did not change significantly (Figure S10). Although we observed embryo-to-embryo variation —this despite scaling stripe phenotypes relative to adjacent stripes in the same embryo— the MSE produces a “weaker” stripe 2 than either WT or INV_MSE, as evidenced by a comparison of relative activation (Figure 5C, p = 0.0114). The INV_MSE appears to have a stripe of intermediate height.
At the late blastoderm stage, MSE and WT both produce a well-differentiated stripe: nearly identical values of relative repression signify equal repression of the anterior and posterior borders (Figure 5D). In contrast, INV_MSE appears to have a derepressed anterior stripe 2 border since it has lower values of relative repression (Figure 5D). Although the WT and INV_MSE distributions are not significantly different at this timepoint (p = 0.1321), the temporal dynamics of INV_MSE relative repression support the conclusion that the anterior border is derepressed (see below). These distinct molecular defects belie the similarities between the two minimal enhancers with respect to both viability and En patterning. Although MSE and INV_MSE are both functional, they are not entirely orientation independent. More careful analysis of the temporal dynamics of stripe formation, described below, reinforces this conclusion.
Dynamics of stripe maturation
Differences in the molecular phenotypes of MSE and INV_MSE compared to WT in late blastoderm embryos can be better understood from the dynamics of stripe formation. Imaging of stripes at three-minute temporal resolution during the time when eve stripe maturation occurs, coupled with the ability to synchronize the embryos to the same absolute time-clock, allowed us to investigate how the “mature” eve stripe phenotypes arose (Figure 5E, 5F). Initially, at the first appearance of an individualized stripe 2 (approximately 30 min.), the three enhancers show similarly low relative activation. The distributions of initial appearance times of a discernable stripe are overlapping for the three genotypes at 25°C (Figure 6A, p = 0.0558 and p = 0.0875, when WT is compared to MSE and INV_MSE respectively). This early similarity in stripe 2 morphology suggests that initial Eve stripe 2 is not dependent on either of the two Hb binding sites contained in the deleted sequences (Figure 1B). However, shortly after the emergence of stripe 2, the maturation process takes on distinct developmental trajectories for the three versions of the enhancer. In particular, over the 18-minute timespan of stripe maturation at 25°C, relative activation of stripe 2 steadily increases in WT, decreases in MSE, and remains nearly constant in INV_MSE. MSE is defective, therefore, in its ability to activate WT levels of stripe 2 gene expression. The dependence of the stripe 2 enhancer on the Hb binding sites for dynamic activation is consistent with the upregulation of Hb expression during cycle 13 and early cycle 14 [36].
Another defect in stripe formation dynamics can be seen with respect to MSE's ability to repress expression in creating the anterior border of stripe 2. In particular, whereas in WT the anterior border grows steadily deeper through the maturation process, evidenced by increasing relative repression (Figure 5F), in MSE the anterior border is overrepressed initially and there is no change over time. A third pattern is seen for the INV_MSE, which exhibits a deepening anterior border, like WT, but at a lower rate. The net consequence of slow INV_MSE peak height and anterior border growth is a visibly derepressed anterior stripe border (Figure 4).
Variability in the initial appearance of stripe 2
The sequences removed in creating the MSE transgene include two footprinted Kr binding sites, kr-2 and kr-1. The Kr repressor is expressed in a broad domain in the middle of the early embryo, its anterior boundary of expression establishing the posterior border of Eve stripe 2 [30], [54]. Based on the results presented so far, kr-2 and kr-1 binding sites are neither essential to S2E function, nor are they required for the placement of the Eve posterior stripe 2 boundary, which doesn't differ from WT. Examination of the temporal dynamics of stripe formation, however, identifies a large difference between MSE and WT in the early formation of stripe boundaries (Figure 5F).
To investigate the early steps in stripe emergence, we used our temporally resolved data in individual embryos to ask the following question: As the early gradient-like expression pattern of Eve resolves into a discernable nascent stripe, does either the anterior or the posterior border of stripe 2 always form first (Figure 7A, 7B)? In 15 WT embryos examined (Figure 7C), we found that this trait varied from embryo to embryo: the anterior border formed first in five embryos, while the posterior border formed first in eight embryos (two embryos could not be resolved). These data confirm, in vivo, a result from an analysis of Eve expression in fixed tissue that the order and manner of stripe formation is variable during early cycle 14 [36]. Since gap gene expression levels have large embryo-to-embryo variability at this stage, variation in the order of initiation of Eve border formation may be a direct readout of these fluctuations.
The anterior and posterior borders form by repression by Gt and Kr respectively [30], [31], [32], [54] and we further hypothesized that embryo-to-embryo variation in the expression levels of these two repressors causes the variable temporal order of stripe 2 border creation. If true, we can predict that if kr-2 and kr-1 are functional, their absence in MSE would make this enhancer less sensitive to the repressive effects of Kr, and as a consequence it would not exhibit as strong a bias as WT towards forming the posterior border first. Consistent with this prediction, we observed a ∼2∶1 anterior border-first bias in MSE (Figure 7C) compared to ∼2∶3 ratio in WT. We conclude from these observations that the variation in the manner of stripe 2 emergence is driven by embryo-to-embryo variation in gap gene expression levels, and that the readout of this variation is sensitive to the presence or absence of the sequences missing in the MSE. INV_MSE shows a greater posterior-first bias than WT, foreshadowing the later derepression of its anterior border.
Precision of stripe placement
Variation in the initiation of the anterior and posterior borders of Eve stripe 2 in WT is temporally resolved to create stereotypical stripe 2 borders. Temporal reduction in positional error is, in fact, a general characteristic of gap and pair-rule expression [36], [56]. In this section we ask whether positional noise in Eve stripe 2 characteristics differ between WT and the MSE. To address this question, we plotted the standard deviations (SD) of estimated locations of the anterior, posterior, and peak positions of stripe 2 as a function of time (Figure 8). Plotting the SD rather than relative positional error is appropriate, as the positions of the peak and borders do not differ between WT, MSE and INV_MSE (Figure S10). As expected, positional variation either remained constant (position of 2A) or decreased over time (position of 2P and peak position), consistent with previous observations [36]. In contrast, all three positional errors increased over time in MSE, leading to a stripe 2 that becomes positionally more variable as it matures. The three traits remained relatively constant for INV_MSE. Since the experimental error arising from sources such as embryo orientation, variable excitation, and background fluorescence is constant in time, any time-dependent effect on positional variance must originate in the intrinsic biological variation of stripe 2 expression. We interpret these results as indicating that sequences contained in the regions deleted in the MSE are required for reducing the variance in Eve stripe 2 positional expression. The other stripe 2 maturation phenotypes, relative activation and repression, did not differ in their variances (Figure S11).
Response to temperature perturbation
As a final experiment, we investigated stripe 2 formation in embryos raised at two developmental temperatures, 25°C and 29°C, focusing on the WT and MSE genotypes. The rationale for the experiment is that the two temperatures will create heterochrony in the rates of development. For example, the impact on the diffusion rates of transcription factors is expected to be much smaller than the impact on enzymatic processes [57], including the ones involved in setting the nuclear division rate. Indeed, the length scale of the Bcd gradient, determined by both transport and enzymatic processes, is strongly affected by temperature [34], and nuclear divisions occur much more rapidly at higher temperatures [45]. The question we address here is: Do the WT and MSE enhancers respond differently to developmental temperature perturbation?
Development is considerably more rapid at 29°C. The mean time at which the cell membrane reaches the basal end of nuclei (Figure S12) is 31 min. compared to 38 min at 25°C, and gastrulation begins around 40 versus 48 minutes.
The results of a previous study suggest that the eve expression pattern scales with developmental time [45], by which we mean that when developmental markers are used to determine time, the Eve expression pattern is qualitatively unchanged upon the application of temperature perturbation. Since we can measure the dynamics of Eve expression quantitatively in absolute time, our data allow us to test temporal scaling. Our data support temporal scaling at a qualitative level, however we found quantitative differences suggesting that the WT pattern at 29°C lags behind the one at 25°C (Figure 9A, 9B). This lag could be due to a differential effect of temperature on YFP maturation versus embryonic development and needs further investigation. Our conclusions below do not depend on a particular assumption about temporal scaling (Figure S13).
We assayed the same phenotypes described in the previous section. An emergent stripe 2 is detectable much earlier in MSE at 29°C than at 25°C (Figure 6, p = 0.0022), whereas WT stripe initiation times are unchanged (p = 0.2392). Similarly, the manner of stripe 2 appearance is perturbed in MSE but not WT. WT maintained its ∼2∶3 posterior-first bias, while MSE switched from a ∼2∶1 anterior-first bias to a ∼2∶3 posterior first bias at 29°C (Figure 9C).
Next, we compare the stripe 2 maturation phenotypes. Given the quicker rate of development at 29°C, we were able to directly compare relative activation and repression time-series (Figure 9A, 9B) at four overlapping time-points. With expression driven by WT, the temporal progression of stripe 2 activation (Figure 9A) is very similar to the one at 25°C. Normalized stripe 2 expression is indistinguishable at the overlapping time-points (p>0.5). MSE, however, drives a pattern of activation at 29°C that is both qualitatively and quantitatively different from the one at 25°C. There is a 14-23% reduction in expression level with statistical significance being achieved at 30 and 33 min (p<0.005).
The relative repression of the borders of the stripe 2 behaves rather differently from activation. Neither WT nor MSE appear to be perturbed at 29°C (Figure 9B, p>0.1798). Similar to its behavior at 25°C, MSE is over-repressed at 29°C.
Discussion
Eukaryotic enhancers are often structurally compact, characterized by the presence of multiple tightly spaced transcription factor binding sites. Apparently redundant binding sites are present not just within the bounds of empirically-defined minimal enhancers, but also in surrounding genomic regions that are not typically included in reporter assays. However, the redundancy of such binding sites, that is, the sufficiency of the minimal enhancer for biological function, has not yet been firmly established.
In a rigorous experimental test to determine whether an empirically defined eukaryotic minimal enhancer —the eve stripe 2 MSE— is biologically active, we found that it could indeed direct gene expression to engage a normal progression of pattern formation, and produce a fully viable fly when homozygous. The MSE is thus biologically sufficient; it is also essential because when deleted (in eveΔMSE), only a rudimentary stripe 2 is formed, en stripe 4 is not produced, and embryonic lethality results. Our experiments establish, therefore, that a minimal enhancer is both necessary and sufficient for biological activity.
This conclusion notwithstanding, MSE and INV_MSE are not fully functional because a single copy of either minimal enhancer transgene in hemizygotes strongly reduced embryonic viability (compared to WT) and produced measurable En patterning defects which could be traced to specific patterning defects in Eve stripe 2 expression. This led us to challenge the enhancer with different genetic backgrounds and temperatures, uncovering a role for the peripheral binding sites in directing robust gene expression.
Our experiment with developmental temperature perturbation shows that MSE stripe establishment and maturation dynamics are temperature sensitive. The WT enhancer, in contrast, responds stereotypically to a range of environmental temperatures (25°C and 29°C are both within the range of temperatures experienced by D. melanogaster embryos [58]). The complete sequence in WT, besides providing compensation to temperature, is also necessary for the precise placement stripe 2 borders.
The sensitivity of MSE to genetic, environmental, and intrinsic sources of variation expressed at multiple levels of development implies that the structure and composition of the WT enhancer are optimized for robust performance. Wildtype enhancer structure therefore, including the peripheral binding sites investigated here, must have an important functional role among natural populations, which are subject to a large amount of genetic and environmental variability.
The temporal reduction of individual-to-individual variation [36], [42] was the first molecular evidence of developmental canalization [59], [60]. Earlier work has identified specific regulatory interactions, occurring in trans, that lead to the canalization of gap gene expression [56], [61]. Here we find that developmental canalization of eve stripe 2 expression is also baked into the architecture of the enhancer itself. Due to the divergent effect of gap gene variation on stripe 2 emergence in MSE, we hypothesize that enhancers have evolved the ability to integrate across variability in the upstream signals to which they respond to assure a stereotypical output.
Under this hypothesis, natural selection is expected to continuously tinker with its structural organization to assure that the enhancer functions across the natural range of input factor variability —stochastic, genetic, and environmental. Hence we propose that adaptive fine-tuning of enhancers to perform robustly may be a force driving binding site turnover, a process recently shown to be influenced by positive selection in Drosophila enhancers [25]. Such a process might explain why the S2E can experience rapid sequence divergence between closely related species, and yet also exhibit functional convergence across much larger evolutionary timescales [26], [62].
Transcriptional networks employ several distinct tactics to ensure reliable outcomes. Some of these act in trans, such as feedback [61], [63] and microRNAs [64], [65], [66], [67], while others, including the role of CRE architecture demonstrated here, act in cis: polymerase stalling [68], redundant enhancers [69], [70], [71], and nucleosome depletion [72]. The multiplicity of mechanisms that contribute to robustness but are otherwise dispensable may have evolved to buffer specific perturbations rather than to offer redundancy. Enhancer structure, for example, might filter extrinsic variation in the concentrations of upstream TFs whereas having redundant enhancers is a strategy to reduce the intrinsic noise of transcription by boosting transcription rate. However, it is also possible that the effect of these mechanisms on core function is not detectable by present methods but is sufficient to provide selective advantage at the population level. Core function and robustness would not be entirely separable if that is the case.
Our study was designed to investigate whether the structural features of an eukaryotic enhancer might contribute directly to the robustness of gene expression, as discussed above, but in the course of the study we also found two indications of developmental canalization acting in subsequent stages of development. One of them is the loss of viability in MSE (or INV_MSE) hemizygotes that is largely masked in homozygotes, which we interpret as a manifestation of the segmentation system's capacity to buffer certain stripe 2 defects. Developmental canalization acting downstream of eve may also explain the buffering of a sex-dependent difference in Eve stripe 2 expression that we also discovered in the course of this study [73]. Contrary to the general belief that segmentation is sex-independent, Eve stripe 2 expression is in fact sex-specific during cycle 14 in both WT and eve+ embryos [73]. MSE hemizygotes have a strong sex-specific effect on viability (and En patterning) not seen in WT, which implies that sequences contained in WT, but eliminated in MSE, are required for the eventual symmetric segmentation between males and females. Further analysis of the sex-specific Eve stripe 2 phenotype implicated the dosage of gt, which being X-linked is present in one copy in males and two copies in females. Lott et al. [74] were the first to investigate whether zygotic expression of genes in the early blastoderm showed evidence of dosage compensation prior to the establishment of the conventional dosage compensation mechanism, and discovered that some genes, including gt, appeared to be compensated. We were able to demonstrate using genetic analysis that the sex-dependent Eve stripe 2 phenotype is dependent on gt dosage [73], implying that the dosage compensation of gt must be incomplete. That a difference in Eve stripe 2 expression in males and females is corrected at a subsequent step in development can be taken as additional evidence for the segmentation system's ability to canalize variation in expression arising earlier in development, in this case originating from sex-chromosome linkage of gt.
Some, but not all stripe 2 phenotypes in MSE and INV_MSE could be rationalized by the elimination of known Hb and Kr binding sites, including the reduction of peak expression (Hb loss) and the delayed initiation of the posterior border (Kr loss) in MSE. Other phenotypes cannot be readily understood, and considering the differences between stripe 2 formation in MSE and INV_MSE, may be dependent on the specific interaction with factors in neighboring sequences. Evolutionary geneticists have long wondered whether the abundance of large chromosomal inversions between species would be a harbinger for a similar abundance of undetected micro-inversions. Enhancers, after all, are supposed to function with orientation independence. Genome sequence comparison among Drosophila species now shows that this is not the case, as the synteny of functional elements within noncoding regions is, in fact, strongly conserved [62], [75]. Our exploration of phenotypic differences between MSE and INV_MSE may provide functional explanation for why noncoding synteny is an evolutionarily conserved trait.
We now return to the question of the physical definition of a cis-regulatory element: Do they have sharply defined boundaries? We think not despite the fact that our experiments fall short of a proof. If enhancers were truly discrete, one would imagine that activator occupancy would change discontinuously at the margins. Since there are measurable effects upon the removal of peripheral sequences, we imagine instead that occupancy decays continuously as one moves away from the empirically defined “core”. Due to the promiscuity of transcription factor binding, this occupancy distribution might extend well beyond the conventional boundaries of the core enhancer and will change with tissue and time. Environmental and genetic perturbation will also change the relative weights of the core and periphery. The evolutionary process of binding site turnover, in turn, ensures that enhancers maintain stereotypical output across a wide range of conditions.
Materials and Methods
Relative viability
Each transgenic rescue line was crossed into the eveR13 (R13) mutant background, generating flies of the genotype w; b,R13 /CyO; attP2[S2EA1EVEA2]/TM3,Sb. A1 refers to the wildtype (wt), MSE or INV_MSE alleles of the stripe 2 enhancer (S2E) and A2 to two alleles of eve coding region, native or tagged with YFP. F1 adults were scored for 2nd and 3rd chromosome phenotypic markers (Cy, b, and Sb), to identify the relevant transgene rescue genotypes (Figure 2A). Replicate crosses were established between 10 females and 20 males in two large culture vials at 25°C. Parents were transferred to a fresh culture vial every day for 20 days. The emerging adult offspring were collected every day from the culture vials for a period of 10 days for scoring. This approach ensured that mutants with slow development rates were counted.
Relative viability of flies carrying one or two copies of the eve transgene and lacking a functional endogenous eve gene was determined from the number of adult survivors. Expected viability for these genotypes was calculated based on the count of flies carrying one copy of the endogenous eve locus and either one or two copies of the transgene-bearing third chromosome (Figure 2A, R13/CyO; attP2[S2EA1EVEA2]/TM3,Sb and R13/CyO; attP2[S2EA1EVEA2], respectively). Employing this procedure, we estimated the relative viability of four different transgene genotypes: 16.4 kb eve without (EVE) and with (WT) the YFP fusion and 16.4 kb eve with YFP fusion carrying either the MSE (MSE) or INV_MSE (INV_MSE) enhancer. In all four cases, the observed ratios of the two genotypes carrying one copy of the endogenous eve locus and either one or two copies of a transgene conformed to the expected 2∶1 segregation ratio (Tables S1 and S2), implying wildtype viabilities for both. On this basis, the numbers of adults produced by these two genotypes were combined to calculate the expected numbers for the rescue transgene genotypes. The comparison of relative viabilities of WT, MSE and INV_MSE versions of the transgene is predicated on the assumption, therefore, that the two genotypes carrying one copy of the native eve locus and one or two copies of the specific transgene are fully viable, a reasonable assumption given that all three stripe 2 enhancer transgenes alone rescued flies to adulthood when homozygous (as described in the Results).
To evaluate the ability of the transgenes to rescue R13, Df(2R)eve (Df(eve)), or eveΔMSE lethality when present in one copy, we crossed eight healthy females of the genotype w; b,R13 /CyO, or w; Df(eve)/CyO, or w; eveΔMSE/CyO, with 15 healthy males of the genotype w; b,R13; attP2[S2EA1EVEA2] in large vials at 25°C. Scoring of emerging adult offspring was as described above.
Constructs
WT, MSE and INV_MSE constructs (Figure 1B; sequences in Text S1) were created by recombineering with Red/ET counter-selection BAC Modification Kit (Gene Bridge http://www.genebridges.com/gb/pdf/K002_Counter_Selection_Kit-V3.0-2007.pdf). The BAC R06J01 was used as the DNA source for the genomic eve locus.
eve-containing DNA, from -6.6 kb to +9.8 (Figure 1A), was cloned into attB_3xP3_DsRed_P15A-Amp by recombineering (vector sequence and primers are provided in Text S1). This eve-containing DNA fragment is slightly larger then the fragments EGN84 (−6.4 kb to +8.4 kb), EGN86 (−6.4 kb to +8.6 kb), and EGN92 (−6.4 kb to +9.2 kb) previously used in rescue assays [47], [50]. The rescue potencies of EGN84, EGN86, and EGN92 have varied, depending on place of transgene insertion in genome, but never exceeding 40% homozygous rescue. The choice of our fragment, -6.6 kb to +9.8, was motivated by the desire to maximize the span of eve-containing DNA bounded by the neighboring genes CG12134 and TER94 and to include experimentally identified endogenous insulator regions (http://www.modencode.org/). This was possible because the recombineering method does not require restriction sites.
The eve-YFP fusion construct was also created by recombineering (primers and sequences are provided in the Text S1). The SYFP2 superfolder, a rapidly maturing version of YFP (generously provided by Ben Glick, University of Chicago), was added to the C-terminus of the eve peptide. The half-life of maturation of the SYFP2 in yeast is ∼8–10 min at 30C (Ben Glick, personal communication).
Structure of altered S2E enhancers
The S2E (798bp) is bordered on the 3′ and 5′ sides by completely conserved blocks of 18bp and 26bp, respectively (marked as blocks a and b in Figure 1B; [27]), which are the generally accepted boundaries of the enhancer. The footprinted binding sites for upstream transcription factors have been described [31], [76]. To create the MSE we deleted two fragments, 33bp and 211bp long, from the distal and proximal regions of S2E respectively (shown as rectangles in Figure 1B). The classic MSE (Minimal Stripe 2 Element) contains 480bp [32]; our MSE adds an additional 29bp distally to avoid the fusion of two repressor binding sites, kr-6 and kr-3, in the INV_MSE construct. This additional native sequence does not contain any mapped TFBS. The 509bp-long MSE and INV_MSE both lack two Kr binding sites (kr-1 and kr-2) and two Hb binding sites (hb-2 and hb-1) and both are bordered by identical sequences. kr-1 and kr-2 are evolutionarily conserved among all species in the melanogaster subgroup [27]. hb-2 differs by only one change between D. melanogaster and D. picticornis, indicating that this sequence must be functionally constrained [27]. In contrast, hb-1 is a relatively young binding site that is present in D. melanogaster and emerged within the melanogaster subgroup [26], [27]. We considered substituting a random sequence for the deleted sequences, but decided against this course of action to avoid the unintended creation of binding sites for unknown TFs.
The attB vector for integration
We created a novel docking site integration vector, the 3265 bp-long attB_3xP3_DsRed_P15A-amp (sequence in Text S1). The compact size of the vector facilitated its amplification by PCR, a necessary step in recombineering. The vector contains an attB sequence for integration, a fly transformation marker, DsRed, expressed in the eye by the PAX-6 promoter, and the p15A origin of replication site that aids in cloning large fragments (up to 50 kb).
Site-specific integration of attB for plasmids into attP2 landing site
Site-specific integration was carried out by co-injection with phiC31-integrase RNA as described [48], [49]. The attP2 D. melanogaster stock was provided by M. Markstein. Integration of the vector attB into the attP2 landing site was verified by using two pairs of primers (see Text S1). The choice of the docking attP2 site was according to [49].
Drosophila strains
Df(2R)eve, eveR13, and eveΔMSE. Df(2R)(eve) is a deficiency that includes at least five lethal complementation groups [77], [78]. The R13 is null mutation that truncates the protein within the homeodomain [47]. We created the eveΔMSE lethal mutant by replacing the 480bp fragment corresponding to the MSE from the endogenous eve locus with the white+ gene using ends-out homologous recombination according to the methods described in [79], [80], [81]. DNA fragments homologous to approximately 4 kb and 3.5 kb of the eve sequences flanking the MSE were cloned into the pTV2 vector. The donor DNA construct was transformed into the germline of Drosophila melanogaster by P-element-mediated germ line transformation [82].
All three lethal mutations were balanced over the marked balancer chromosome CyO, p[hb-lacZ] to allow the identification of mutant embryos by immunostaining for β-galactosidase or by PCR analysis for the β-galactosidase gene. PCR-based genotyping of individual Drosophila embryos after immunostaining is described in [26]. Also, the R13 null mutant was balanced over the fluorescently marked balancer chromosome CyO,p[Dfd-YFP] to allow the identification of mutant larvae.
Analysis of embryos in fixed tissue
Embryo collection and fixation was as described [83]. Drosophila embryos were immunostained with Rabbit polyclonal anti-Eve (provided by Mark Biggin, University of California, Berkeley, 1∶1,000 dilution) and Chicken polyclonal anti-GFP (abcam, USA, 1∶3,000 dilution) primaries and Alexa Fluor-546, Alexa Fluor-647 Goat anti-Rabbit IgG (Molecular Probes, Invitrogen, 1∶400 dilution), and Alexa Fluor-647 goat anti chicken IgG (Molecular Probes, Invitrogen, 1∶400 dilution) secondaries.
Histochemical staining with anti-En monoclonal 4D9 at 1∶10 dilution was visualized using HRP-DAB enhanced by nickel [83].
in situ hybridization was carried out as described [27], [42].
Live imaging
We recombined the attP2[S2EA1EVEYFP] and P[His2Av-mRFP1] (Bloomington stock 23650) transgenes onto the same third chromosome to visualize Eve-YFP and nuclei in parallel. Due to the low fertility of the recombinant homozygous genotype, we imaged embryos from a cross between attP2[S2EA1EVEYFP] males and attP2[S2EA1EVEYFP],P[His2Av-mRFP1]/TM3,Sb females. The His-RFP fluorescence observed in cleavage cycle 14 is primarily maternal since mRFP1 matures slowly. As a result, we imaged individual embryos carrying either one or two copies of Eve-YFP. We could make comparisons between lines and treatments because we always normalized stripe 2 expression levels to that of stripe 1 (Figure 4B) or the anterior border height to that of the posterior border (Figure 5A).
We maintained flies at a constant temperature, either 25C or 29C, and collected embryos on apple juice plates for 1–1.5 hours. The embryos were allowed to age for another hour before being dechorionated in 50% bleach for 3.5 min. The embryos were then mounted on circular coverslips for a temperature control chamber (FCS3, Bioptechs Inc., Butler, PA, USA). We oriented the embryos laterally by hand and placed a drop of 700 series Halocarbon oil such that embryos at the edge of the drop were partially exposed to air. The chamber was mounted on the microscope stage and heated to the target temperature. The objective was also heated to ensure a uniform and stable temperature distribution. The period of time for which the embryos were at room temperature, during dechorionation and mounting, was not more than 15 min.
We observed a significant attenuation of YFP signal in embryos completely covered by Halocarbon oil, although their development appeared normal. This is consistent with the quenching of GFP fluorescence in anaerobic conditions [55]. For this reason we only chose embryos that were partially exposed to air for imaging.
We identified a cycle 13 embryo and observed it in the histone channel, undergoing the thirteenth nuclear division. To allow a comparison of embryos in absolute time, we started the clock during the final mitotic wave [84] from telophase to cycle 14 interphase. This wave is identifiable by the presence of cycle 14 interphase nuclei at the poles and telophase nuclei at the equator of the embryo. On average mitotic waves last 0.5 min [84], allowing us to determine the age of each embryo during imaging within ±0.5 min. After this point, we imaged the embryo at the midsagittal plane every 3 min for an hour, when gastrulation movements begin.
Confocal microscopy
We imaged embryos using a Vti Infinity 3 multipoint confocal system (Visitech International, Sunderland, UK) mounted on a Zeiss AxioPlan 2 microscope (Carl Zeiss, Inc., USA). A backthinned EMCCD camera (Hamamatsu Photonics UK Ltd, Hertfordshire, UK) having a resolution of 512x512 pixels and 16 bit depth was employed for fluorescence detection.
For YFP, excitation was provided by a 514 nm solid state laser with a triple band (442 nm, 514 nm, 633 nm) dichroic. A dual band (450–490 nm and 515–580 nm) emission filter was used for detection. mRFP1 emission is less than 10% of peak for wavelengths less than 580 nm, minimizing crosstalk. The 561 nm laser line, a dual band dichroic (420 and 560 nm) and 585 nm long pass emission filter were used for detecting mRFP1.
The frequency of image acquisition (every 3 min) and exposure time (2–5 sec) were chosen conservatively to minimize photobleaching and maximize signal to background ratio. At this frequency of acquisition, we observed signal attenuation with time only at an exposure of 10 sec. With a 2–5 sec exposure, the brightest embryos had a few pixels at the maximum detection limit of the camera. All embryos within a set of experiments (either 25C or 29C) were acquired with the same microscope settings.
Image segmentation
We adapted an algorithm used to segment images of immunofluorescently-stained flattened embryos [85] for use with live image data from the midsagittal plane. The original algorithm works in two steps, 1) a whole embryo mask is used to rotate, orient, and crop the image and 2) after smoothing, the watershed algorithm is applied to separate the nuclei and make a nuclear mask.
We made two modifications that enable fully automated segmentation save for the user input required in orienting the embryo. First, instead of a whole embryo mask we create a cortical mask since yolk autofluorescence leads to spurious detection of nuclei. We use the gray-scale top-hat transformation [86] followed by Otsu thresholding to remove yolk autofluorescence. Next, erosions followed by morphological reconstruction on the thresholded binary image remove the autofluorescent vittelline membrane. Second, we correct oversegmentation caused by the invaginating cell membrane during the middle of cycle 14. We compute the neighbors of each watershed region. A pair of watershed regions is considered to belong to the same nucleus if 1) they are separated by a watershed line greater than one pixel in length and 2) one region touches the yolk but not the outside while the other touches the outside and not the yolk. The members of such pairs are then fused. The mean Eve-YFP fluorescence is calculated in the mask corresponding to each nucleus and is saved along with the coordinates of the centroid for further processing.
Feature detection
We used the CSAPS function of MATLAB (MathWorks Inc.) to determine a smoothed cubic spline approximation to the fluorescence data. Given data vectors x and y, CSAPS determines a spline, f(x), that minimizes a cost function that is a sum of the total error made by the spline in approximating the data and a measure of the ‘roughness’ of the spline. The relative weight of these two terms is controlled by the roughness parameter p. p = 1 yields a perfect, but non-smooth, fit, whereas p = 0 gives a least-squares straight line fit to the data. We chose a value, p = 0.5, to give a good fit without detecting spurious extrema and used the same value for all embryos. The mean error of the spline approximation at the extrema was ∼10% at this value of p.
The spline was used to estimate the positions and fluorescence levels at the extrema in each embryo (Figure 5B). Border positions were calculated as the position where the fluorescence level is at the mean of the consecutive extrema. The height of a border is the difference in fluorescence levels at consecutive extrema.
In order to determine which border formed first (Figure 7A, 7B), we used the spline to follow the temporal evolution of the Eve pattern (Video S1). In each embryo, we noted the order in which the minima immediately anterior and posterior to the stripe 2 peak were first detected by the spline. We ensured that these minima were genuine by following them through time and confirming that they developed into mature interstripes.
Supporting Information
Zdroje
1. SchaffnerW 1999 Enhancer. CreightonT The Encyclopedia of Molecular Biology New York John Wiley and Sons, Inc. 823 828
2. PennacchioLARubinEM 2001 Genomic strategies to identify mammalian regulatory sequences. Nat Rev Genet 2 100 109
3. LudwigMZ 2002 Functional evolution of noncoding DNA. Curr Opin Genet Dev 12 634 639
4. PierstorffNBergmanCMWieheT 2006 Identifying cis-regulatory modules by combining comparative and compositional analysis of DNA. Bioinformatics 22 2858 2864
5. HeXLingXSinhaS 2009 Alignment and prediction of cis-regulatory modules based on a probabilistic model of evolution. PLoS Comput Biol 5 e1000299 doi:10.1371/journal.pcbi.1000299
6. SuJTeichmannSADownTA 2010 Assessing computational methods of cis-regulatory module prediction. PLoS Comput Biol 6 e1001020 doi:10.1371/journal.pcbi.1001020
7. ArnoneMIDavidsonEH 1997 The hardwiring of development: organization and function of genomic regulatory systems. Development 124 1851 1864
8. SodergrenEWeinstockGMDavidsonEHCameronRAGibbsRA 2006 The genome of the sea urchin Strongylocentrotus purpuratus. Science 314 941 952
9. BermanBPNibuYPfeifferBDTomancakPCelnikerSE 2002 Exploiting transcription factor binding site clustering to identify cis-regulatory modules involved in pattern formation in the Drosophila genome. Proc Natl Acad Sci U S A 99 757 762
10. BermanBPPfeifferBDLavertyTRSalzbergSLRubinGM 2004 Computational identification of developmental enhancers: conservation and function of transcription factor binding-site clusters in Drosophila melanogaster and Drosophila pseudoobscura. Genome Biology 5 R61
11. ErivesALevineM 2004 Coordinate enhancers share common organizational features in the Drosophila genome. Proc Natl Acad Sci U S A 101 3851 3856
12. HalfonMSGradYChurchGMMichelsonAM 2002 Computation-based discovery of related transcriptional regulatory modules and motifs using an experimentally validated combinatorial model. Genome Res 12 1019 1028
13. LiLZhuQHeXSinhaSHalfonMS 2007 Large-scale analysis of transcriptional cis-regulatory modules reveals both common features and distinct subclasses. Genome Biol 8 R101
14. BergOGvon HippelPH 1987 Selection of DNA binding sites by regulatory proteins. Statistical-mechanical theory and application to operators and promoters. J Mol Biol 193 723 750
15. StormoGD 2000 DNA binding sites: representation and discovery. Bioinformatics 16 16 23
16. TanayA 2006 Extensive low-affinity transcriptional interactions in the yeast genome. Genome Res 16 962 972
17. JanssensHHouSJaegerJKimARMyasnikovaE 2006 Quantitative and predictive model of transcriptional control of the Drosophila melanogaster even skipped gene. Nat Genet 38 1159 1165
18. SegalERaveh-SadkaTSchroederMUnnerstallUGaulU 2008 Predicting expression patterns from regulatory sequence in Drosophila segmentation. Nature 451 535 540
19. KazemianMBlattiCRichardsAMcCutchanMWakabayashi-ItoN 2010 Quantitative analysis of the Drosophila segmentation regulatory network using pattern generating potentials. PLoS Biol 8 e1000456 doi:10.1371/journal.pbio.1000456
20. HardingKHoeyTWarriorRLevineM 1989 Autoregulatory and gap gene response elements of the even-skipped promoter of Drosophila. The EMBO Journal 8 1205 1212
21. SmallSBlairALevineM 1996 Regulation of two pair-rule stripes by a single enhancer in the Drosophila embryo. Developmental Biology 175 314 324
22. McGregorAPOrgogozoVDelonIZanetJSrinivasanDG 2007 Morphological evolution through multiple cis-regulatory mutations at a single gene. Nature 448 587 590
23. SchroederMDPearceMFakJFanHUnnerstallU 2004 Transcriptional control in the segmentation gene network of Drosophila. PLoS Biol 2 e271 doi:10.1371/journal.pbio.0020271
24. MosesAMPollardDANixDAIyerVNLiXY 2006 Large-scale turnover of functional transcription factor binding sites in Drosophila. PLoS Comput Biol 2 e130 doi:10.1371/journal.pcbi.0020130
25. HeBZHollowayAKMerklSJKreitmanM 2011 Does positive selection drive transcription factor binding site turnover? A test with Drosophila cis-regulatory modules. PLoS Genet 7 e1002053 doi:10.1371/journal.pgen.1002053
26. LudwigMZPalssonAAlekseevaEBergmanCMNathanJ 2005 Functional evolution of a cis-regulatory module. PLoS Biol 3 e93 doi:10.1371/journal.pbio.0030093
27. LudwigMZPatelNHKreitmanM 1998 Functional analysis of eve stripe 2 enhancer evolution in Drosophila: rules governing conservation and change. Development 125 949 958
28. GotoTMacDonaldPManiatisT 1989 Early and late periodic patterns of even-skipped expression are controlled by distinct regulatory elements that respond to different spatial cues. Cell 57 413 422
29. StanojevicDHoeyTLevineM 1989 Sequence-specific DNA-binding activities of the gap proteins encoded by hunchback and Krüppel in Drosophila. Nature 341 331 335
30. SmallSKrautRHoeyTWarriorRLevineM 1991 Transcriptional regulation of a pair-rule stripe in Drosophila. Genes and Development 5 827 839
31. StanojevicDSmallSLevineM 1991 Regulation of a segmentation stripe by overlapping activators and repressors in the Drosophila embryo. Science 254 1385 1387
32. SmallSBlairALevineM 1992 Regulation of even-skipped stripe 2 in the Drosophila embryo. The EMBO Journal 11 4047 4057
33. ArnostiDNBaroloSLevineMSmallS 1996 The eve stripe 2 enhancer employs multiple modes of transcriptional synergy. Development 122 205 214
34. HouchmandzadehBWieschausELeiblerS 2002 Establishment of developmental precision and proportions in the early Drosophila embryo. Nature 415 798 802
35. GregorTTankDWWieschausEFBialekW 2007 Probing the limits to positional information. Cell 130 153 164
36. SurkovaSKosmanDKozlovKManuMyasnikovaE 2008 Characterization of the Drosophila Segment Determination Morphome. Developmental Biology 313 844 862
37. ElowitzMBLevineAJSiggiaEDSwainPS 2002 Stochastic gene expression in a single cell. Science 297 1183 1186
38. BlakeWJKaernMCantorCRCollinsJJ 2003 Noise in eukaryotic gene expression. Nature 422 633 637
39. AriasAMHaywardP 2006 Filtering transcriptional noise during development: concepts and mechanisms. Nature Reviews Genetics 7 34 44
40. EldarADorfmanRWeissDAsheHShiloBZ 2002 Robustness of the BMP morphogen gradient in Drosophila embryonic patterning. Nature 419 304 308
41. EldarAElowitzMB 2010 Functional roles for noise in genetic circuits. Nature 467 167 173
42. LottSEKreitmanMPalssonAAlekseevaELudwigMZ 2007 Canalization of segmentation and its evolution in Drosophila. Proc Natl Acad Sci U S A 104 10926 10931
43. MilesCMLottSEHendriksCLLudwigMZManu 2010 Artificial selection on egg size perturbs early pattern formation in Drosophila melanogaster. Evolution 65 33 42
44. CheungDMilesCKreitmanMMaJ 2011 Scaling of the Bicoid morphogen gradient by a volume-dependent production rate. Development 138 13 2741 9
45. LucchettaEMLeeJHFuLAPatelNHIsmagilovRF 2005 Dynamics of Drosophila Embryonic Patterning Network Perturbed in Space and Time Using Microfluidics. Nature 434 1134 1138
46. ForceAGCreskoWAPickettFB 2004 Information Accretion, Gene Duplication, and the Mechanisms of Genetic Module Parcellation. SchlosserGWagnerGP Modularity in Development and Evolution Chicago University of Chicago Press 315 337
47. FujiokaMEmi-SarkerYYusibovaGLGotoTJaynesJB 1999 Analysis of an even-skipped rescue transgene reveals both composite and discrete neuronal and early blastoderm enhancers, and multi-stripe positioning by gap gene repressor gradients. Development 126 2527 2538
48. GrothACFishMNusseRCalosMP 2004 Construction of transgenic Drosophila by using the site-specific integrase from phage phiC31. Genetics 166 1775 1782
49. MarksteinMPitsouliCVillaltaCCelnikerSEPerrimonN 2008 Exploiting position effects and the gypsy retrovirus insulator to engineer precisely expressed transgenes. Nat Genet 40 476 483
50. FujiokaMYusibovaGLPatelNHBrownSJJaynesJB 2002 The repressor activity of Even-skipped is highly conserved, and is sufficient to activate engrailed and to regulate both the spacing and stability of parasegment boundaries. Development 129 4411 4421
51. Nüsslein-VolhardCKludingHJurgensG 1985 Genes affecting the segmental subdivision of the Drosophila embryo. Cold Spring Harbor Symposiums on Quantitative Biology 50 145 154
52. GregorTWieschausEFMcGregorAPBialekWTankDW 2007 Stability and nuclear dynamics of the Bicoid morphogen gradient. Cell 130 141 152
53. InghamPWBakerNEMartinez-AriasA 1988 Regulation of segment polarity genes in the Drosophila blastoderm by fushi-tarazu and even-skipped. Nature 331 73 75
54. FraschMHoeyTRushlowCDoyleHJLevineM 1987 Characterization and localization of the Even-skipped protein of Drosophila. The EMBO Journal 6 749 759
55. HeimRPrasherDCTsienRY 1994 Wavelength mutations and posttranslational autoxidation of Green Fluorescent Protein. Proc Natl Acad Sci U S A 91 12501 12504
56. ManuSurkovaSSpirovAVGurskyVVJanssensH 2009 Canalization of gene expression and domain shifts in the Drosophila blastoderm by dynamical attractors. PLoS Comput Biol 5 e1000303 doi:10.1371/journal.pcbi.1000303
57. SegelIH 1975 Enzyme Kinetics. New York John Wiley & Sons
58. FederMECartanoNVMilosLKrebsRALindquistSL 1996 Effect of engineering Hsp70 copy number on Hsp70 expression and tolerance of ecologically relevant heat shock in larvae and pupae of Drosophila melanogaster. J Exp Biol 199 1837 1844
59. WaddingtonCH 1942 Canalization of development and the inheritance of acquired characters. Nature 150 563 565
60. WaddingtonCH 1959 Canalization of development and genetic assimilation of acquired characters. Nature 183 1654 1655
61. ManuSurkovaSSpirovAVGurskyVVJanssensH 2009 Canalization of gene expression in the Drosophila blastoderm by gap gene cross regulation. PLoS Biol 7 e1000049 doi:10.1371/journal.pbio.1000049
62. HareEEPetersonBKIyerVNMeierREisenMB 2008 Sepsid even-skipped Enhancers Are Functionally Conserved in Drosophila Despite Lack of Sequence Conservation. PLoS Genet 4 e1000106 doi:10.1371/journal.pgen.1000106
63. AcarMPandoBFArnoldFHElowitzMBvan OudenaardenA 2010 A general mechanism of network-dosage compensation in gene circuits. Science 329 5999 1656 1660
64. AmbrosV 2004 The functions of animal microRNAs. Nature 431 350 355
65. BartelDP 2004 MicroRNAs: Genomics, Biogenesis, Mechanism, and Function. Cell 116 281 297
66. GaulU 2010 Decoding transcription and microRNA-mediated translation control in Drosophila development. Biol Chem 391 767 770
67. LiXCassidyJJReinkeCAFischboeckSCarthewRW 2009 A microRNA imparts robustness against environmental fluctuation during development. Cell 137 273 282
68. BoettigerANLevineM 2009 Synchronous and stochastic patterns of gene activation in the Drosophila embryo. Science 325 471 473
69. FrankelNDavisGKVargasDWang SPayreF Phenotypic robustness conferred by apparently redundant transcriptional enhancers. Nature 466 490 493
70. PerryMWBoettigerANBothmaJPLevineM 2010 Shadow enhancers foster robustness of Drosophila gastrulation. Curr Biol 20 1562 1567
71. PerryMWCandeJDBoettigerANLevineM 2009 Evolution of insect dorsoventral patterning mechanisms. Cold Spring Harb Symp Quant Biol 74 275 279
72. BarriereAGordonKLRuvinskyI 2011 Distinct functional constraints partition sequence conservation in a cis-regulatory element. PLoS Genet 7 e1002095 doi:10.1371/journal.pgen.1002095
73. ManuLudwigMZKreitmanM 2011 Sex-specific pattern formation during early Drosophila development. Proc Natl Acad Sci U S A In review
74. LottSEVillaltaJESchrothGPLuoSTonkinLA 2011 Noncanonical compensation of zygotic X transcription in early Drosophila melanogaster development revealed through single-embryo RNA-seq. PLoS Biol 9 e1000590 doi:10.1371/journal.pbio.1000590
75. RanzJMMaurinDChanYSvon GrotthussMHillierLW 2007 Principles of genome evolution in the Drosophila melanogaster species group. PLoS Biol 5 e152 doi:10.1371/journal.pbio.0050152
76. AndrioliLPMVasishtVTheodosopoulouEObersteinASmallS 2002 Anterior repression of a Drosophila stripe enhancer requires three position-specific mechanisms. Development 129 4931 4940
77. O'BrienMARobertsMSTaghertPH 1994 A genetic and molecular analysis of the 46C chromosomal region surrounding the FMRFamide neuropeptide gene in Drosophila melanogaster. Genetics 137 121 137
78. GoldsteinESTreadwaySLStephensonAEGramstadGDKeiltyA 2001 A genetic analysis of the cytological region 46C-F containing the Drosophila melanogaster homolog of the jun proto-oncogene. Mol Genet Genomics 266 695 700
79. GongWJGolicKG 2003 Ends-out, or replacement, gene targeting in Drosophila. Proc Natl Acad Sci U S A 100 2556 2561
80. GongWJGolicKG 2004 Genomic deletions of the Drosophila melanogaster Hsp70 genes. Genetics 168 1467 1476
81. RongYSGolicKG 2001 A targeted gene knockout in Drosophila. Genetics 157 1307 1312
82. RubinGMSpradlingAC 1982 Genetic transformation of Drosophila with transposable element vectors. Science 218 348 353
83. PatelNHCondronBGZinnK 1994 Pair-rule expression patterns of even-skipped are found in both short- and long-germ beetles. Nature 367 429 434
84. FoeVEAlbertsBM 1983 Studies of nuclear and cytoplasmic behaviour during the five mitotic cycles that precede gastrulation in Drosophila embryogenesis. The Journal of Cell Science 61 31 70
85. JanssensHKosmanDVanario-AlonsoCEJaegerJSamsonovaM 2005 A high-throughput method for quantifying gene expression data from early Drosophila embryos. Dev Genes Evol 215 374 381
86. GonzalezRCWoodsRE 2002 Digital image processing. Upper Saddle River, NJ, USA Prentice-Hall Inc.
Štítky
Genetika Reprodukční medicínaČlánek vyšel v časopise
PLOS Genetics
2011 Číslo 11
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