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.2024 Mar 7;20(3):e1011204.
doi: 10.1371/journal.pgen.1011204. eCollection 2024 Mar.

Cis-regulatory polymorphism at fiz ecdysone oxidase contributes to polygenic evolutionary response to malnutrition in Drosophila

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Cis-regulatory polymorphism at fiz ecdysone oxidase contributes to polygenic evolutionary response to malnutrition in Drosophila

Fanny Cavigliasso et al. PLoS Genet..

Abstract

We investigate the contribution of a candidate gene, fiz (fezzik), to complex polygenic adaptation to juvenile malnutrition in Drosophila melanogaster. Experimental populations maintained for >250 generations of experimental evolution to a nutritionally poor larval diet (Selected populations) evolved several-fold lower fiz expression compared to unselected Control populations. Here we show that this divergence in fiz expression is mediated by a cis-regulatory polymorphism. This polymorphism, originally sampled from a natural population in Switzerland, is distinct from a second cis-regulatory SNP previously identified in non-African D. melanogaster populations, implying that two independent cis-regulatory variants promoting high fiz expression segregate in non-African populations. Enzymatic analyses of Fiz protein expressed in E. coli demonstrate that it has ecdysone oxidase activity acting on both ecdysone and 20-hydroxyecdysone. Four of five fiz paralogs annotated to ecdysteroid metabolism also show reduced expression in Selected larvae, implying that malnutrition-driven selection favored general downregulation of ecdysone oxidases. Finally, as an independent test of the role of fiz in poor diet adaptation, we show that fiz knockdown by RNAi results in faster larval growth on the poor diet, but at the cost of greatly reduced survival. These results imply that downregulation of fiz in Selected populations was favored by selection on the nutritionally poor diet because of its role in suppressing growth in response to nutrient shortage. However, they suggest that fiz downregulation is only adaptive in combination with other changes evolved by Selected populations, which ensure that the organism can sustain the faster growth promoted by fiz downregulation.

Copyright: © 2024 Cavigliasso et al. This is an open access article distributed under the terms of the Creative Commons Attribution License, which permits unrestricted use, distribution, and reproduction in any medium, provided the original author and source are credited.

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Conflict of interest statement

The authors have declared that no competing interests exist.

Figures

Fig 1
Fig 1. Genomic and expression differentiation offiz gene between Control (C1-C6) and Selected (S1-S6) populations.
A. Positions and allele frequencies at candidate SNPs in the genomic vicinity offiz relative to gene transcripts. Allele frequencies are estimated from pooled whole genome sequencing [18]; for each SNP the frequency plotted is that of the allele more frequent in the Selected than in Control populations. All Selected populations are (nearly) fixed for one allele at all SNPs, and four Control populations are fixed for the alternative allele. Only SNPs assessed as significantly differentiated between Selected and Control populations are plotted; for a full list of polymorphisms in this region see S1 Table. B. Expression offiz in third instar larvae raised on the poor diet, based on previously published RNAseq data [11,19]. The values are averages from the two conditions used in that study (germ free andAcetobacter-inoculated); the expression in the two conditions was highly correlated across populations (r = 0.99).CG14406 is a gene of unknown function immediately upstream offiz; it is not differentially expressed between Selected and Control populations (P = 0.75).
Fig 2
Fig 2. In vitro activity of purified Fiz protein on ecdysone and 20E.
A and B. Production of H2O2 by Fiz protein incubated with ecdysone (A) and 20E (B) as substrates, compared to Fiz protein alone or substrate alone, in relative units. C and D. Reduction of the relative concentration of ecdysone (C) and 20E (D) following incubation with Fiz protein. Bars correspond to the means ± SE of N = number of replicate reactions; “+” and “-” indicate the presenceversus absence of a particular compound.
Fig 3
Fig 3
(A) Relative expression of focal genes in third instar larvae raised on standard diet (means ± SE from qPCR relative to three reference genes). (B) Timing of the sampling points relative to larval development (white and black bars indicate the light and darkness periods). 3.5-day-old L2 larvae were collected, those that molted to L3 overnight were collected next morning ("early L3"), with further samples taken 24h and 36h later. For each gene and diet, thePreg andPreg×stage refer to the main effect of the evolutionary regime (i.e., Selected versus Control) and to regime × stage interaction, respectively. Asterisks indicate a significant stage-specific pairwise difference between Control and Selected populations afterP-value correction (sequential Bonferroni adjustment for stages).N = 3 populations × 3 replicates of 10 pooled larvae per evolutionary regime and stage.
Fig 4
Fig 4. Expression of alleles offiz andCG9512 in F1 crosses between Control and Selected populations.
A,B: Proportional contribution of the "Selected" allele to the transcript pool offiz (A) andCG9512 (B) in heterozygous F1 female larvae, determined by amplicon sequencing. The proportion of the "Selected" allele in 50:50 mix of cDNA from parental lines provides a reference. C,D: Relative expression (from RT-qPCR) offiz andCG9512 in F1 male larvae (hemizygous for both X chromosome genes) compared to the parental populations. SEL: Selected; CTL: Control; F1 crosses are represented as maternal × paternal population. The three symbols per category correspond to three independent population pairs (C2 × S1, C4 × S2, C6 × S3). Each symbol indicates mean ± SE of N = 2 to 4 (A-B) or 4 (C-D) replicates per population or cross; each replicate consisted of a pool of seven late third instar larvae. ***P < 0.001, n.s.P > 0.05.
Fig 5
Fig 5. Effect of ubiquitousfiz RNAi knockdown on egg-to-adult survival probability (A), developmental time (B), female weight (C) and estimated female growth rate (D) on poor and standard diets.
Symbols indicate means ± SE.N = 4 replicate bottles for poor and 5 bottles for standard diet (each bottle initially contained 200 eggs). Red and blue lines in C and D represent predictions from statistical models (including the linear and quadratic components).
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This work was supported by the Swiss National Science Foundation (grants 31003A_162732 and 310030_184791 to TJK) and by funding from the University of Lausanne. The funders had no role in study design, data collection and analysis, decision to publish, or preparation of the manuscript.

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