Alternative splicing, muscle contraction and intraspecific variation: associations between troponin T transcripts, Ca2+ sensitivity and the force and power output of dragonfly flight muscles during oscillatory contraction
208 Mueller Laboratory, Department of Biology, Pennsylvania State University, University Park, PA 16802, USA
*e-mail: jhm10{at}psu.edu
Accepted July 23, 2001
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Summary |
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Key words: dragonfly, insect flight muscle, work loop, skinned fiber, Ca2+ sensitivity, cooperativity, troponin T, alternative splicing, Libellula pulchella.
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Introduction |
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How alternative splicing of RNA affects function at the subcellular and cellular levels is becoming increasingly well understood (Baker et al., 2001; Pilotte et al., 2001), for example, as are ways in which the precise control of RNA splicing affects cell fate and organogenesis (e.g. sex determination in Drosophila) (Lopez, 1998). Alternative splicing may be one of the primary mechanisms underlying phenotypic plasticity and acclimation yet, curiously, relationships between ribotypic variation and continously variable organismal traits have received scant attention. It is also likely that there is heritable variation in the regulation of alternative splicing within populations, in which case the identity and evolution of alternative-splicing-regulating genes should be a topic of interest for population and evolutionary biology.
Here, we present a study that examines the relationship between ribotypic variation and a continuously variable trait and how ribotypes and trait values differ among populations and morphs. Specifically, we relate intraspecific variation in transcript composition of the troponin T (TnT) gene with intraspecific variation in the contractile performance of dragonfly flight muscles. Dragonflies hunt, defend territories and mate aerially, and their flight muscle contractile performance is therefore likely to have a powerful effect on virtually all aspects of their adult biology and reproductive fitness.
Unlike many insects that have asynchronous, stretch-activated flight muscles (Josephson et al., 2000), dragonflies have synchronous flight muscles in which each contraction is initiated by a neural stimulus (Simmons, 1977b), with no evidence for stretch activation. Neural stimulation causes release of Ca2+ from the sarcoplasmic reticulum, which then binds with the troponin complex on the thin filament to initiate cross-bridge binding, an increase in tension and muscle shortening (Ohtsuki, 1999). We have shown in previous work that one of the three troponin subunits, troponin T (TnT), exists as multiple isoforms in the flight muscles of Libellula pulchella dragonflies, that ontogenetic variation in TnT isoform expression is correlated with changes in isometric twitch tension, whereas tetanic tension and unloaded shortening velocity are age-invariant (Fitzhugh and Marden, 1997), and that the mixture of TnT alternative transcripts is significantly related to variation in wing kinematics during free flight, which in turn affects aerial performance and the energetic cost of flight (Marden et al., 1999).
Because insect flight muscles operate at high contraction frequencies, the mediation of activation and relaxation by the troponin complex is likely to play an especially important role. At high contraction frequencies, the transition phase between activation and relaxation constitutes a high proportion of the total contraction cycle, and steady-state conditions are probably never attained. The work-loop technique (Josephson, 1985; Stevenson and Josephson, 1990) was developed for the purpose of assessing muscle contractile performance under realistic stress, strain and stimulation regimes, in which the non-steady-state characteristics of contraction can be observed and quantified. Here, we use the work-loop technique to determine how variation in the relative abundance of TnT transcripts is related to contractile function during a reasonable approximation of in vivo working conditions. The results contribute to our goal of developing an integrative understanding of muscle physiology and locomotor performance in this species (Marden et al., 1998) and, more generally, to knowledge of how molecular and cellular variation affect the complex in vivo mechanics of muscle contraction (Lutz and Lieber, 2000; Wakeling et al., 2000). We also explore ontogenetic and population differences in alternative splicing of TnT. Our findings highlight the need for population and evolutionary studies of processes that control alternative splicing, in addition to more commonly examined types of allelic variation [e.g. (Watt, 1992; Harrison et al., 1996; Powers and Schulte, 1998)].
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Materials and methods |
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Tissue preparation and RNA analysis
Following completion of experiments with intact muscle (described below), approximately half the total flight musculature from each dragonfly was flash-frozen and stored in liquid nitrogen, or at 70°C, for use in TnT isoform profiling. Additional tissue was placed in isotonic buffer solution (as described by Marden et al., 1999) with 1 % Triton X-100 and glycerol, and kept at 20°C. This tissue was stored for up to 2 weeks prior to determination of skinned fiber Ca2+ sensitivity.
A fluorescent labeling technique (Luehrsen et al., 1997) was used to quantify the relative abundance of different TnT transcripts in the flight muscle of individual dragonflies (Wolf, 1999; Marden et al., 1999). RNA was recovered from muscle samples using RNAqueous (Ambion, Austin, TX, USA) and reverse-transcribed to first-strand cDNA (Boehringer-Mannheim). TnT cDNAs were amplified using primers that span the alternatively spliced region. The forward primer, located in the 5' untranslated region, was fluorescently labeled with 6fam dye (5'-6fam CGCTTCTTTCACTCGTTGTTCAAAC-3'). The reverse primer (5-CCTTCGCTTGGCTTGCTTC-3') was located in a constitutive exon downstream (3') from the alternatively spliced region. The amplified TnT fragments were separated on an ABI 377 automated sequencer (Applied Biosystems) and quantified according to the amount of fluorescence detected (GeneScan 2.1; Applied Biosystems).
We used the peak heights from the GeneScan profiles to determine the relative quantity of each TnT fragment. Our measures of transcript relative abundance show qualitative agreement with protein isoform composition determined from two-dimensional gels and western blots (Marden et al., 1999); this agrees with results from other studies that have found that the relative abundances of alternatively spliced TnT transcripts correspond closely to the abundances of the protein isoforms they encode (Mesnard-Rouiller et al., 1997). Thus, we assume that variation among individuals in relative abundance of different TnT transcripts is a reasonably accurate measure of variation in TnT protein isoforms within the flight muscles.
Relative quantities of each isoform were arcsine-transformed prior to statistical analyses (Sokal and Rohlf, 1995). All statistical analyses were performed with JMP software (SAS Institute).
Ca2+ sensitivity
Measurements of the Ca2+ sensitivity of force generation by detergent-skinned fibers were obtained as described previously (Marden et al., 1999). These experiments began with a small fiber bundle (mean diameter 53 µm) completely submerged in a chamber containing isotonic relaxing solution (pCa 8) at 25°C. The bundle was held at each end with clamps similar to those described previously (Moss, 1979), one of which was attached to a three-dimensional micromanipulator and the other to a 404A force transducer (Aurora Scientific). Sarcomere lengths were set at 2.32.4 µm (which matches the native sarcomere length determined by fixation of in situ muscle) using a Leica DMIL inverted microscope equipped with a CCD camera and monitor. Relaxing solution was replaced by activating solutions of progressively higher Ca2+ concentration, and isometric tension was measured after equilibration in each activating solution. The Ca2+ sensitivity of the fiber bundle was characterized as the negative logarithm of the Ca2+ concentration producing half-maximal tension (pCa50). The Hill cooperativity coefficient (nH) was determined from an iterative fit of the Hill equation.
Determination of the in vivo contractile regime
The wingbeat frequencies and amplitudes used by L. pulchella during high-performance free flight [upper quartiles 36 Hz and 68° for a sample of 59 escape flights; data from (Marden et al., 1999)] are also exhibited during high-effort flight attempts by dragonflies attached to a force transducer (Fig. 1B). At maximal effort, the net vertical forces over a number of wingbeat cycles by L. pulchella tethered in this fashion average approximately three times body weight (Marden, 1995), which corresponds with the maximal load that this species can lift during free flight (Marden, 1987). These data indicate that the contractile regime of the flight muscles during bouts of high-effort tethered flight should be a reasonably close approximation to the in vivo working conditions of the muscle during peak effort (excluding quick turns and maneuvers, which have different wingbeat kinematics).
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The distance-calibrated LDS voltage waveform was used to determine the wing angle during flapping (Fig. 1D). From these data and a measurement of the distance between the insertion point of the tendon-like apodeme of the basalar muscle and the wing hinge, we calculated the strain cycle of the basalar muscle during high-exertion flight attempts. We confirmed these estimates by also positioning the laser of the LDS on the humeral plate (Snodgrass, 1935) of the forewing, directly above the insertion point of the basalar muscles apodeme (Fig. 1A). Both methods estimated the peak-to-peak distance variation of the basalar muscle to be approximately 0.52 mm during high-amplitude flapping. This value is approximately 10 % of the resting length of the basalar muscle (mean basalar muscle length 5.4 mm).
EMG electrodes were inserted approximately 1 mm apart, midway along the length of the basalar muscle. Voltage spikes followed a slow time course (approximately 5 ms rise time; Fig. 2A) and had variable amplitudes; these features are characteristic of both intracellular and extracellular recordings from dragonfly motor neurons and flight muscles (Fig. 2B) [data from (Simmons, 1977b)], which do not fire conventional all-or-none action potentials.
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The slow time course of electrical events in dragonfly flight muscles made it difficult to determine the in vivo phase relationship between the precise onset of stimulation and muscle strain. Thus, in preliminary work-loop experiments, we varied the stimulus onset in a series of 1 ms steps so that it occurred at seven different points on the strain cycle (Fig. 3). The stimulus phase onset that optimized net work during contraction at 37 Hz was approximately 22 % of the total strain cycle (i.e. at 44 % of the lengthening portion of the cycle). We used this stimulus phase in subsequent experiments.
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Muscle temperature was monitored with a fine-gauge thermocouple implanted in the center of the thorax. The contractile performance of some preparations began to degrade between initial tests at 28°C and the target test temperature of 32°C; degradation consisted of a marked increase in passive tension accompanied by a decrease in active tension. To avoid reductions in sample size, we analyzed, for each individual, the series of contractions at any temperature between 28 and 32°C that produced the highest power output, and we included temperature as a variable in our statistical analyses. Most of the muscle preparations deteriorated rapidly at temperatures greater than 3234°C. Our total sample consisted of one basalar muscle from each of 21 individual dragonflies.
Analog output from a computer was used to drive the lever and the attached basalar muscle through a series of oscillations that corresponded to 10 % strain at integer frequencies from 20 to 45 Hz. The computer program (a macro written in Igor; Wavemetrics Inc.) triggered a single electrical stimulus of 0.25 ms duration (determined in preliminary experiments to be the minimal stimulus duration required to evoke maximal twitch tension). Five contraction cycles were measured at each frequency; we analyzed the fourth cycle from each of these sets. At each frequency, we also recorded tension during a strain cycle that lacked a stimulus; the resulting trace of passive tension was overlaid on the trace of active tension at that frequency to determine the time of onset of active force.
Net work output was measured from the area enclosed by counterclockwise-progressing work loops, minus any area within clockwise-progressing portions (i.e. the product of net force and distance) (Josephson, 1985); the product of net work and frequency yielded mechanical power output. To quantify variability in the shape of work loops, we measured the following variables at several contraction frequencies (20, 24, 27, 30, 34, 37, 40 and 44 Hz): the time of onset of active force, peak force, force at 50 % of the shortening phase and the time from 50 % of peak activation to 50 % relaxation (i.e. half-width of activation). Fig. 4 illustrates these variables. For measures involving only the magnitude of forces, we have normalized for a small amount of variation in resting tension (mean 0.6 N cm2) by subtracting the minimum force measured for each cycle from the active forces; the reported force measurements are therefore net forces.
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Results |
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Both morphs undergo a two- to threefold increase in body mass during adult maturation. This mass increase consists primarily of internal growth of flight muscle and ovaries (Marden, 1989). The extent of maturation for an individual can be quantified by relating body mass to a maturationally invariant exoskeletal dimension. For this purpose, we use residuals from the regression of the cube root of body mass on forewing length as an index of relative maturity. Dragonflies belonging to the early morph showed a significant relationship between relative maturity and the Ca2+ sensitivity of muscle activation (Fig. 7A; r2=0.64, P<0.0001), whereas the late morph showed no such relationship (Fig. 7B; r2=0.0002, P=0.85). The relative abundance of TnT 267 also increased significantly with relative maturity in the early morph (r2=0.26, P=0.02) but not in the late morph (r2=0.17, P=0.10), whereas the relative abundance of TnT 261 increased significantly with relative maturity in both morphs (r2>0.4, P<0.004 in both morphs). Thus, distinct subpopulations follow different ontogenetic trajectories for certain aspects of alternative splicing and muscle contractile physiology.
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Work per cycle
Work output at 37 Hz averaged 2.4 J kg1, with a range of 0.734.0 J kg1. In univariate models, specific work was positively related to the relative abundance of TnT 267 (r2=0.54; P<0.0001; Fig. 8) and to Ca2+ sensitivity (r2=0.45; P=0.0005). Neither of these relationships varied among morphs (P>0.74 in both cases). In a stepwise regression analysis that included Ca2+ sensitivity, the relative abundance of TnT 267, the relative abundance of TnT 261, temperature, morph and the Hill coefficient (log-transformed to achieve normality) as independent variables, only the relative abundance of TnT 267 (partial r2=0.53; P=0.0004) and temperature (partial r2=0.09; P=0.07) had significant or marginally significant effects on specific work.
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The same set of independent variables, either alone or in multivariate combinations, failed to explain a significant proportion of the variation in the location of peak force or the half-width of activation (percentage of the contraction cycle over which force was at least 50 % of maximal). In general, these results show little effect of the measured variables on the timing of muscle activation and deactivation (although temperature certainly has a large effect when varied over a larger range).
Magnitude of force production
The peak net force developed during work-loop contractions at 37 Hz varied between 3.0 and 11.0 N cm2. Ca2+ sensitivity (r2=0.53, P<0.0001) and the relative abundances of both TnT 261 (r2=0.42, P=0.002) and TnT 267 (r2=0.35, P=0.005) each showed strong positive relationships with peak net force in univariate linear regressions. However, these are not independent effects since these variables were significantly correlated with each other. Only the relative abundance of TnT 261 had a significant effect when all three of these variables were included in a single linear model. The model that appears to best describe the variation in peak force is a quadratic fit based on the pooled relative abundance of TnT 261 and TnT 267 (r2=0.74, P=0.0001; Fig. 10). The significant second-order term in this relationship (P=0.0003) suggests that the highest observed levels of these generally force-enhancing TnT isoforms are associated with a decline in force production.
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Power output
There was a wide range of variation among individual muscles in their maximum specific power output (the highest power output recorded across all contraction frequencies; 45155 W kg1; Fig. 12, Fig. 13). As we found for peak work-loop force, a large proportion of this variation was explained in univariate models both by the pooled relative abundance of TnT 261 and TnT 267 (r2=0.48, P=0.0005; Fig. 13A) and by Ca2+ sensitivity (r2=0.51, P=0.0001; Fig. 13B). Using both these independent variables in a multivariate model resulted in essentially no increase in explanatory power (r2=0.55) and, although the overall model was highly significant, neither of these independent variables showed a significant effect independently of the other. Thus, one or both of these independent variables are correlated with maximum power output, and our data do not distinguish any differences in their effects.
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Optimum cycle frequency
Temperature had a weak effect on the optimal frequency for power output (i.e. the contraction frequency at which maximum power was produced; r2=0.28, P=0.01); this effect becomes much more pronounced when temperature is varied over a wider range than we used in the present experiments. Ca2+ sensitivity, the Hill coefficient and the individual or pooled relative abundance of any TnT transcripts did not explain any of the remaining variation in optimal frequency. This result is consistent with our observation (see above) that the independent variables examined in this study had little effect on the timing of muscle activation.
Differences in contractile performance between populations
In addition to the physiological differences that we observed among morphs (Fig. 7), there were significant differences in the mean values from our two study ponds for nearly every biochemical and physiological variable that we measured (Table 2). Our data also suggest that there may be population differences in some of the relationships between physiological variables. For example, the quadratic fit that we show in Fig. 10 may hide what is actually a positive linear relationship between the relative abundance of TnT 261 and TnT 267 and force production in the Ten Acre Pond population and a negative linear relationship or no relationship between these variables in the Mothersbaugh population. For most of our data, there is a relatively small range of variation for the independent variable within the Mothersbaugh population, which makes it difficult to determine whether this population shows a different relationship or simply presents too little statistical leverage to detect the trend. Without more data showing the effects of low levels of Ca2+ sensitivity or the relative abundance of TnT 261 in the Mothersbaugh population, it is impossible to resolve this question. The only exception to this problem is the relative abundance of TnT 267, which had a nearly equal range of variation in the two populations; here, we see an identical relationship in both populations (Fig. 8, Fig. 11).
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Discussion |
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Two features of our correlative results strengthen the likelihood that TnT variation has a causal role in these relationships. First, the two distinct morphs of L. pulchella undergo different ontogenetic patterns of Ca2+ sensitivity, power output and the relative abundance of one particular TnT transcript, yet these morphs are indistinguishable in all comparisons involving the relationship between TnT transcript abundances and physiological variables. Thus, we can reject the hypothesis that changes in TnT splicing are simply a marker for physiological changes related to age or maturation. Second, we found a strong relationship between the relative abundance of a particular TnT transcript (267) and a particular aspect of contraction (force per cross-sectional area midway through the shortening phase; Fig. 11). The relative abundance of TnT 267 is correlated with that of other TnT transcripts as well as with Ca2+ sensitivity, yet none of these other variables shows nearly as strong a relationship with force midway through the shortening phase.
A number of experimental manipulations of TnT have produced results that demonstrate a strong effect of TnT variation on muscle contractile performance. Changing TnT content, most commonly by introduction of a transgene carrying a point mutation, has been shown to cause changes in Ca2+ sensitivity, force and cross-bridge cycling rates in single filaments, actomyosin solutions and cultured muscle cells (Tobacman and Lee, 1987; Sweeney et al., 1998; Watkins et al., 1996; Chandra et al., 1999; Nakaura et al., 1999; Purcell et al., 1999; Rust et al., 1999; Homsher et al., 2000). One study has shown that the ratio of mutant to wild-type troponin T protein has strong effects on contractility (Redwood et al., 2000); this result is quite similar to what we found for the ratio of naturally occurring alternative transcripts. Transgenic mice carrying mutant forms of cardiac TnT have consistently shown changes in systolic and/or diastolic function of their intact hearts, as well as changes in Ca2+ sensitivity of cardiac skinned fibers (Oberst et al., 1998; Tardiff et al., 1999; Frey et al., 2000; Knollmann et al., 2001; Miller et al., 2001). Generally, transgenic experiments have found that mutated forms of TnT cause an increase in Ca2+ sensitivity, force and cross-bridge cycling rates, i.e. the mutation has disrupted the normal modulatory effect of TnT on muscle contractility.
The transgenic studies discussed above have used point mutations that cause amino acid replacements at regions of the molecule that are not affected by alternative splicing. Experimental manipulations of TnT have not yet begun to examine the functional effects of variability in TnT that arise from ubiquitous alternative splicing at the 5' end of the molecule. The study that comes closest is that of Chandra et al. (Chandra et al., 1999), who replaced native TnT with an amino-terminal truncated version of TnT (TnT-trunc). TnT-trunc interacted more strongly with tropomyosin, which stabilized contractile filaments in a submaximally activated state. That result demonstrates that the amino terminal of TnT serves to weaken the binding affinity between TnT and tropomyosin, and thereby reduces the inhibition of myosin cross-bridge attachment [for a similar result, see (Ogut and Jin, 2000)]. Thus, the strong relationship between the abundance of TnT transcripts and muscle activation and force production in dragonflies is presumably caused, at least in part, by differences in the way TnT protein isoforms affect the troponin/tropomyosin interaction that regulates muscle activation. Although our correlative data leave open the possibility that other molecular changes are involved, the studies cited above indicate that TnT alone is capable of causing the observed effects. If so, then variation in the ratio of alternatively spliced TnT isoforms may be a particularly potent mechanism for varying contractile mechanics, since small changes in the relative abundance of a fairly rare transcript, TnT 267, are associated with large changes in contractile performance.
A key mechanistic question is how variation in muscle contractile performance affects wingbeat kinematics and flight performance. Wakeling and Ellington (Wakeling and Ellington, 1997a; Wakeling and Ellington, 1997b) have performed detailed studies of wingbeat kinematics of a libellulid dragonfly and found that the stroke plane is rigidly fixed at 48° from the longitudinal body axis and that variation in only two variables, wingbeat amplitude and frequency, explained more than 90 % of a 4.5-fold range of variation (35156 W kg1) in their calculation of muscle mass-specific aerodynamic power output (we obtained this result by combining data from their two papers). In a separate study (Marden et al., 1999), we have shown that the TnT transcript mixture (expressed as the first principal component of variability among the relative abundances of all TnT transcripts) is significantly related to the wingbeat frequency of L. pulchella dragonflies during free flight.
Our current results allow us to reanalyze those data in a more specific fashion, since we now know that particular TnT transcripts are strongly associated with contractile performance. This reanalysis shows that the relative abundance of both TnT 261 (P=0.03, one-tailed) and TnT 267 (P=0.008, one-tailed) is positively correlated with wingbeat frequency, and that the relative abundance of TnT 261 is positively correlated with wingbeat amplitude (P=0.04, one-tailed). Thus, dragonflies with enhanced muscle contractility appear to increase the amplitude and frequency of their wingbeats. This is somewhat at odds with the results of our contractile experiments, in which our data explained a large proportion of the variation in peak force and work per cycle, but little or none of the variation in the timing of force onset or optimal contraction frequency. However, it must be kept in mind that our experiment examined the force output of muscles undergoing invariant externally imposed strain and stimulation regimes, whereas an intact animal can freely vary its strain and stimulation regime on the basis of many forms of mechanical and sensory feedback. One hypothesis is that greater muscle force should create higher wing accelerations and velocities, which should in turn cause increased wingbeat frequency. Precisely how the contractile differences that we report in the present study relate to wingbeat kinematics and aerial performance remains an open question.
We have previously presented fairly detailed discussions of the possible ecological benefits of dragonflies being able to modulate their muscle power output, flight performance and energetic costs over a wide range (Marden et al., 1998; Marden et al., 1999). Rather than repeat those arguments, which are not substantially changed by our new data, we will concentrate here on the new observation that dragonflies from different ponds show significant differences in the mean power output of their flight muscles and that morphs within ponds show different maturational trends in muscle contractile physiology. Presumably, alternative splicing of TnT is a phenotypically variable trait, which responds within individual dragonflies to changes in physical conditions (i.e. energy storage levels, frequency and intensity of flight) and social variables (i.e. crowding and the intensity of territorial interactions). Modulation of muscle contractile performance may allow dragonflies to operate at different points along a trade-off between aerial performance and energetic cost (Marden et al., 1999), and therefore it is perhaps not surprising to find that dragonflies from different ponds have made this adjustment differently. Differences in the maturational pattern of variability in muscle contractility among morphs may reflect either different environments during the fairly distinct seasons when the two morphs are present as adults or it may reflect fixed differences in the internal hormonal environments of early- versus late-emerging dragonflies. At present, these are only hypotheses; the mechanisms and ecological ramifications of these differences among individuals, morphs and populations remain to be determined.
Many studies have examined the whole-organism functional consequences of allelic variation (Barnes and Laurie-Ahlberg, 1986; Barnes et al., 1989; Watt, 1992; Harrison et al., 1996; Powers and Schulte, 1998), but there has been little effort to date to examine how alternative splicing (i.e. non-allelic variation that arises at the RNA level) affects continuous variation in whole-organism traits. One reason for this lack of attention is that alternative splicing can be viewed as simply a mechanism for generating non-heritable phenotypic variation and is thus perhaps of little interest for population or evolutionary biology. However, our demonstration of different patterns of alternative splicing in distinct subpopulations suggests that there may be functionally important variation in the genes and pathways that control alternative splicing. Trans-regulatory genes that control alternative splicing are becoming increasingly well characterized [e.g. (Cooper, 1998; Ladd et al., 2001)], which suggests that there will be opportunities for organismal and population biologists to study these processes that amplify the complexity and phenotypic diversity obtainable from a limited number of genes.
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Acknowledgments |
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