Comparative Cytogenetics of the Malagasy Ground Geckos of the Paroedura bastardi and Paroedura picta Species Groups

Simple Summary Chromosome changes represent important events in evolution. They may trigger processes of speciation or be the result of phylogenetic diversification. In both cases they can represent discrete evolutionary markers of taxonomic significance. In this contribution, we performed a comparative cytogenetic analysis on several representatives of the Malagasy ground geckos of the genus Paroedura. Our results show that chromosome variability in this genus involves chromosome number, morphology, and the independent differentiation of sex chromosome systems in distinct evolutionary lineages. We also highlight that the taxonomic, genetic and chromosome diversity in Paroedura is still underestimated. Abstract We present a comparative chromosome study of several taxa of the Malagasy ground geckos of the Paroedura bastardi and P. picta species groups. We employed a preliminary molecular analysis using a trait of the mitochondrial 16S rRNA gene (of about 570 bp) to assess the taxonomic status of the samples studied and a cytogenetic analysis with standard karyotyping (5% Giemsa solution), silver staining (Ag–NOR staining) and sequential C-banding (C-banding + Giemsa and + fluorochromes). Our results show that all the taxa studied of the P. bastardi group (P. ibityensis, P. rennerae and P. cf. guibeae) have a similar karyotype composed of 2n = 34 chromosomes, with two metacentric pairs (1 and 3) and all other pairs being acrocentric. Chromosome diversification in the P. bastardi group was mainly linked to the diversification of heteromorphic sex chromosome systems (ZZ/ZW) in P. ibityensis and P. rennerae, while no heteromorphic sex chromosome pair was found in P. cf. guibeae. The two taxa investigated of the P. picta species group (here named P. picta and P. cf. picta based on molecular data) showed the same chromosome number of 2n = 36, mostly acrocentric elements, but differed in the number of metacentric elements, probably as a result of an inversion at chromosome pair 2. We highlight that the genus Paroedura is characterized by the independent diversification of heterogametic sex chromosomes in different evolutionary lineages and, similarly to other phylogenetically related gecko genera, by a progressive formation of a biarmed element by means of tandem fusions and inversions of distinct pairs.


Introduction
The complex geological history and geomorphology of Madagascar have resulted in an exceptional environmental variability that is reflected by its highly diversified biomes and zoocoenoses [1].In particular, the herpetofauna of Madagascar comprises an extraordinary diversity at different taxonomic levels and a high rate of endemic and microendemic species [2].Overall, the squamate reptiles of the region include twelve families of snakes (Boidae, Elapidae, Psammophiidae, Pseudoxyrhophiidae, Typhlopidae, and Xenotyphlopidae) and lizards (Agamidae, Chamaeleonidae, Gekkonidae, Gerrhosauridae, Opluridae and Scincidae) with more than 460 described species and several genetic evolutionary lineages that are still awaiting formal description [3].Among the reptile families from Madagascar, the extant representatives of the family Gekkonidae represent a significant fraction of the total squamate diversity of the island, including more than 140 described species that are subdivided into eleven genera (Blaesodactylus, Ebenavia, Geckolepis, Gehyra, Hemidactylus, Lygodactylus, Matoatoa, Paroedura, Paragehyra, Phelsuma, and Uroplatus) [3].With the exception of Lygodactylus (which includes representatives from Southern Africa and South America), Gehyra (which is mostly distributed between Southeast Asia and Oceania) and Hemidactylus (which is one of the most widespread reptile genus worldwide), all other eight gecko genera are endemic to Madagascar and its surrounding islands [4].Among them, the genus Paroedura includes 23 described endemic species of ground geckos from Madagascar and two species from the Comoros [3].The complex taxonomy of the genus has been updated several times in the last few years with the resurrection and the new description of several species [5][6][7][8].
In the first chromosome analyses on the genus, Main et al. [12] and Aprea et al. [13] described the karyotypes of 2 and 11 species, respectively, including several taxa of the P. bastardi and P. picta species groups.These studies show that the genus is characterized by a karyotype composed of 2n = 31-38 mostly acrocentric chromosomes, with NORs always localized on microchromosome pairs and the occurrence of a putative multiple sex chromosome system with female heterogamety (Z 1 Z 1 Z 2 Z 2 /Z 1 Z 2 W) in P. gracilis.Further chromosome studies on the genus have evidenced the presence of simple sex chromosome systems with female heterogamety (ZW) in several species (P.masobe, P. karstophila, P. oviceps, P. stumpffi and P. lohatsara), while a putative multiple sex chromosome system was found in P. gracilis [14].The occurrence of this unusual sex chromosome system in P. gracilis was hypothesized considering the presence of two female-specific heterochromatic elements (W 1 and W 2 ) and an even chromosome complement (2n = 38) in both males and females [14].Interestingly, while the simple sex chromosome system of the first five species was considered to be homologous, the absence of heteromorphic sex chromosomes in some species, as well as the derived multiple sex chromosome system in P. gracilis, led to the hypothesis of their possible secondary loss in some taxa [14,15].
The emerging karyological scenario identifies the genus Paroedura as an excellent study model in evolutionary cytogenetics.In fact, the species so far karyotyped show a significant variability both in terms of chromosome number and morphology, as well as in the diversification of sex chromosomes.However, their taxonomy has been revised since the cytogenetic studies cited above, resulting in a confusing picture.
In this study, we performed a comparative cytogenetic analysis on several representatives of the P. bastardi and the P. picta species groups, reworking some samples previously studied by Aprea et al. [13], providing new karyological data of some taxa and linking the molecular species delimitation recently performed by Miralles et al. [7] and Piccoli et al. [8] to the available karyotype data.
We describe the chromosome formula and the occurrence of putative heterogametic sex chromosome pairs in additional species of the P. bastardi and P. picta species groups, including an undescribed molecular clade from Eastern Madagascar.Our results highlight that the observed genetic and cytogenetic diversity of Paroedura is still underestimated, and that this genus should be the focus of further molecular and cytogenetic studies.Finally, considering the available cytogenetic data, we offer a hypothesis on the karyotype evolution of the P. bastardi and P. picta species groups.

Sampling
Nine individuals of the genus Paroedura from Madagascar were analyzed in this study.The identification numbers, sampling locality, sex of the samples studied as well as their taxonomic attribution after molecular analysis (see below) are listed in Table 1.The samples were collected during fieldwork conducted between 2002 and 2004 by various collaborators and no animal was sampled during the realization of this study.After capture, the individuals were injected with a colchicine solution of 0.5 mg/mL (0.1 mL/10 g of body weight).Tissue samples were then incubated for 30 min in hypotonic solution (KCl 0.075 M + sodium citrate 0.5%, 1:1), and fixed and preserved in Carnoy's solution (methanol/acetic acid, 3:1).The fixed biological material was stored at 4 • C and transferred to the laboratory, where it was processed as described below.The experimental procedures described below were conceived to provide new molecular and chromosome data on the genus Paroedura, also by filling some informational gaps left by Aprea et al. [13] (e.g., missing DNA sequences and/or karyotypes).The taxonomic attribution of the study samples provided in Table 1 was determined by means of a preliminary molecular analysis using a trait of the 16S rDNA (16S) (samples GA324, GA325, GA505, GA388, FGMV1523, FGMV1524) (see below) or using homologous traits previously provided by Aprea et al. [13] (for samples GA506, GA389 and FGMV1522).

Molecular Analysis
We performed a preliminary molecular analysis in order to assess the taxonomic identity of the samples analyzed and to link the available DNA sequences to the newly described karyotypes.In particular, the molecular procedures described as follows were realized on the samples GA 388 and GA 505 (which were not analyzed with molecular methods in Aprea et al. [13]) and on the samples FGMV 1523, FGMV 1524, GA 324 GA 325 (which were not analyzed with either molecular or cytogenetic methods in Aprea et al. [13]).Genomic DNA was extracted from cell suspensions and tissue samples using the standard phenol-chloroform reported in Sambrook et al. [16].
PCR was performed in 25 µL of reaction volume and using the following cycle conditions: an initial denaturation step at 94 • C for 5 min, followed by 36 cycles of denaturation at 94 • C for 30 s, annealing at 55 • C for 30 s, extension at 72 • C for 45 s and a final elongation step at 72 • C for 7 min.The resulting amplicons were then sequenced using the BigDye Terminator 3.1 kit (ABI) and an ABI 377 automated sequencer (Applied Biosystems, Foster City, CA, USA).The chromatograms obtained were visually checked and edited with Chromas Lite 2.6.6 and BioEdit 7.7.1 [19].To perform a molecular taxonomic attribution, all the newly generated DNA sequences were blasted on GenBank and compared with available homologous sequences, previously used in taxonomic and phylogenetic studies on the genus Paroedura [5,[7][8][9]11,13].The sequences with an identity score ≥ 98% (uncorrected p-distance) were considered to be conspecific.

Cytogenetic Analysis
Chromosomes in metaphase were obtained using the air-drying technique as reported by Mezzasalma et al. [20].Metaphase plates were stained with standard methods (10 min in a solution of 5% Giemsa at pH 7), silver (Ag-NOR) staining [21], C-banding as described by Sumner [22] and sequential C-banding + CMA 3 and + DAPI [23].Metaphase plates were scored and recorded by means of an optical and an epifluorescence microscope (Axioscope Zeiss, Oberkochen, Germany) equipped with an image analysis system.The reconstruction of karyotypes and the calculation of the chromosome relative length (RL = chromosome length/total length of the karyotype) and centromeric index of each chromosome (CI = short arm length/total length of the chromosome) were then performed after the acquisition of at least 15 metaphase plates per individual studied, and chromosomes were classified following the categories proposed by Levan et al. [24], as metacentric (m), submetacentric (sm), subtelocentric (st) or acrocentric (a).

Cytogenetic Analysis
The reconstruction of karyotypes with standard staining (5% Giemsa solution at pH 7) was successfully performed on all the samples studied.Our results highlight that the karyotype of all the studied individuals of the P. bastardi species group (P.ibytensis, P. rennerae and P. cf. guibei) (see Table 1) have a similar chromosome formula of 2n = 34 chromosomes, which gradually decrease in size without showing any clear distinction between macroand microchromosome pairs (Figure 1).These species also show a similar chromosome morphology with two metacentric chromosomes (here represented as chromosome pairs 1 and 3), while all the remaining pairs are acrocentric (Figure 1).The female specimens of P. ibytiensis, and P. rennerae showed a dimensionally heteromorphic chromosome pair (here described as chromosome pair 10), which was also more evident after C-banding (see below).No heteromorphic chromosome pair was detected in the male samples of the same species or in P. guibeae (Figure 1).The two specimens of P. picta and P. cf. picta both show a chromosome complement of 2n = 36, mostly composed of acrocentric chromosome pairs that are gradually decreasing in size (Figure 1).However, in P. picta, one chromosome pair is metacentric (pair 3), while in P. cf. picta, two pairs are metacentric (pairs 2 and 3) (Figure 1).No heteromorphic chromosome pair was observed in the studied female samples of P. picta and P. cf. picta (Figure 1).
After Ag-NOR staining, all the studied species of Paroedura showed paired NOR loci on a small chromosome pair (here depicted as the last chromosome pair) (Figure 1).
C-banding and sequential C-banding evidenced a generally low content of heterochromatin in all the studied species (Figures 2 and 3).These species also show a similar chromosome morphology with two metacentric chromosomes (here represented as chromosome pairs 1 and 3), while all the remaining pairs are acrocentric (Figure 1).The female specimens of P. ibytiensis, and P. rennerae showed a dimensionally heteromorphic chromosome pair (here described as chromosome pair 10), which was also more evident after C-banding (see below).No heteromorphic chromosome pair was detected in the male samples of the same species or in P. guibeae (Figure 1).The two specimens of P. picta and P. cf. picta both show a chromosome complement of 2n = 36, mostly composed of acrocentric chromosome pairs that are gradually decreasing in size (Figure 1).However, in P. picta, one chromosome pair is metacentric (pair 3), while in P. cf. picta, two pairs are metacentric (pairs 2 and 3) (Figure 1).No heteromorphic chromosome pair was observed in the studied female samples of P. picta and P. cf. picta (Figure 1).
After Ag-NOR staining, all the studied species of Paroedura showed paired NOR loci on a small chromosome pair (here depicted as the last chromosome pair) (Figure 1).
C-banding and sequential C-banding evidenced a generally low content of heterochromatin in all the studied species (Figures 2 and 3).
Distinct heterochromatic blocks were mostly present on telomeric, centromeric and pericentromeric regions of most chromosome pairs, which, in P. ibityensis, P. rennerae and P. cf. guibeae, were evident with bot C-banding + Giemsa and C-banding + fluorochromes (Figure 2).In P. picta and P. cf. picta, heterochromatic blocks were more evident with C-banding + Giemsa (Figure 3) than with C-banding + fluorochromes.Furthermore, in P. ibytensis and P. rennerae, the small element of the heteromorphic pair 10 proved to be largely heterochromatic, possibly corresponding to the heterogametic chromosome of a sex chromosome pair with female heterogamety (ZW).Interestingly, the W element of P. ibytensis appeared relatively smaller than the W chromosome of P. rennerae (Figures 1 and 2).No heteromophic chromosome was found in P. cf. guibeae (Figure 2) or in P. picta and P. cf. picta (Figure 3).Distinct heterochromatic blocks were mostly present on telomeric, centromeric and pericentromeric regions of most chromosome pairs, which, in P. ibityensis, P. rennerae and P. cf. guibeae, were evident with bot C-banding + Giemsa and C-banding + fluorochromes (Figure 2).In P. picta and P. cf. picta, heterochromatic blocks were more evident with C-banding + Giemsa (Figure 3) than with C-banding + fluorochromes.Furthermore, in P. ibytensis and P. rennerae, the small element of the heteromorphic pair 10 proved to be largely heterochromatic, possibly corresponding to the heterogametic chromosome of a sex chromosome pair with female heterogamety (ZW).Interestingly, the W element of P. ibytensis appeared relatively smaller than the W chromosome of P. rennerae (Figures 1 and  2).No heteromophic chromosome was found in P. cf. guibeae (Figure 2) or in P. picta and P. cf. picta (Figure 3).Distinct heterochromatic blocks were mostly present on telomeric, centromeric and pericentromeric regions of most chromosome pairs, which, in P. ibityensis, P. rennerae and P. cf. guibeae, were evident with bot C-banding + Giemsa and C-banding + fluorochromes (Figure 2).In P. picta and P. cf. picta, heterochromatic blocks were more evident with C-banding + Giemsa (Figure 3) than with C-banding + fluorochromes.Furthermore, in P. ibytensis and P. rennerae, the small element of the heteromorphic pair 10 proved to be largely heterochromatic, possibly corresponding to the heterogametic chromosome of a sex chromosome pair with female heterogamety (ZW).Interestingly, the W element of P. ibytensis appeared relatively smaller than the W chromosome of P. rennerae (Figures 1 and  2).No heteromophic chromosome was found in P. cf. guibeae (Figure 2) or in P. picta and P. cf. picta (Figure 3).

Molecular Analysis
Our molecular results help us to assess the taxonomic status of the specimens of the P. bastardi and P. picta species groups with available cytogenetic data.In particular, we are confident about the taxonomic attribution of P. ibityensis (for samples GA 388 and GA 389) and P. rennerae (for samples GA 505 and GA 506), which showed a sequence identity score > 98% with different specimens that have been recently used in taxonomic and phylogenetic studies on the genus (see [7,8]).In turn, our results on P. cf. guibeae show (also according to the phylogenetic relationships provided in [7]) the existence of distinct molecular clades ascribed to P. guibeae, which probably deserve a focused taxonomic assessment and might represent a species complex.In fact, these different molecular clades (respectively, from Isalo, Tranoroa and Toliara) form three distinct branches in the phylogenetic tree provided by Miralles et al. [7], showing significant haplotype diversity.The specimens analyzed in this study (FGMV 1523 and FGMV 1524), which were also incorporated in the phylogenetic analysis in [7]), belong to the Toliara clade.However, because no molecular data are available for specimens from the type locality of the species (Betroka), it is uncertain which molecular clade corresponds to P. guibeae s.s., and we here prefer to refer to the samples analyzed in this study as P. cf. guibeae.
Interestingly, we also found a significant haplotype diversification between available sequences of P. picta and the samples GA 324 and GA 325, which are here referred to as P. cf. picta, also considering the karyotype differences observed (see Results).We chose to refer to sample FMGV 1522 as P. picta and samples GA 324 and GA 325 as P. cf. picta, considering that the locality reported for the former is geographically closer to the type locality of the species (Madagascar, St. Augustins Bay) [27].

Cytogenetic Analysis
Chromosome data may provide valuable taxonomic and evolutionary information on the taxa studied.In fact, different chromosome characters (e.g., number, morphology, localization of particular chromosome markers and absence/presence of differentiated sex chromosomes) can represent ancestral or apomorphic states, which can be useful to understanding evolutionary dynamics (see e.g., [20,[28][29][30]).
Overall, our results highlight that the karyotype variability in the P. bastardi and P. picta species groups involves chromosome number (2n = 34-36), chromosome morphology (with a different complement of metacentric and telocentric elements) and the independent diversification of ZZ/ZW heterogametic sex chromosome pairs (Figure 4).The three available karyotypes of the P. bastardi group (P.ibityensis, P. rennerae and P. cf. guibeae) all show a similar karyotype with 2n = 34 characterized by two metacentric pairs (1 and 3), which mostly differ by the presence/absence and diversification stage of a ZW heteromorphic chromosome pair (Figure 4).
In fact, a similar putative ZZ/ZW sex chromosome pair was detected in this study in both P. ibityensis and P. rennerae, where the W chromosome appears largely heterochromatic and smaller than the Z chromosome.The relatively smaller size of the W of P. ibityensis (see Results) can be explained by the progressive degeneration of the heterochromatic sex chromosome, which is commonly observed in several evolutionary lineages (see e.g., [31]).It should be noted that the differentiation of heterogametic sex chromosomes in these species was not previously highlighted in Aprea et al. [13], probably because only standard chromosome staining was performed on representatives of those species.In Koubová et al. [14], sex chromosomes were also not reported for P. ibityensis, but as already specified above, the deposited DNA sequence associated to this species corresponds to P. guibeae, which was later resurrected in Miralles et al. [7].Concerning the specimens here identified as P. cf. guibeae, we also did not find any evidence of a differentiated sex chromosome system, thus confirming previous observations and suggesting that sex chromosomes in this species are probably in an early stage of diversification, and mostly pseudo-autosomal.In the P. picta species group, no differentiated sex chromosomes were observed in P. picta or P. cf. picta, but a ZZ/ZW sex chromosome system was reported by Koubová et al. [14] in P. masobe (Figure 4).As previously pointed out in Koubová et al. [14] and Rovatsos et al. [15], different possible explanations can be hypothesized in order to explain the absence/presence of heteromorphic sex chromosome pairs and the occurrence of different stages of diversification in the genus Paroedura.The first hypothesis implies the reversal of differentiated sex chromosomes back to the undifferentiated state (with a possible sex chromosome turnover), while the second accounts for different diversification rates in distinct clades (see [15]).In fact, a similar putative ZZ/ZW sex chromosome pair was detected in this stu both P. ibityensis and P. rennerae, where the W chromosome appears largely hetero matic and smaller than the Z chromosome.The relatively smaller size of the W of tyensis (see Results) can be explained by the progressive degeneration of the h chromatic sex chromosome, which is commonly observed in several evolutionary ages (see e.g., [31]).It should be noted that the differentiation of heterogamet chromosomes in these species was not previously highlighted in Aprea et al. [13], ably because only standard chromosome staining was performed on representati those species.In Koubová et al. [14], sex chromosomes were also not reported for tyensis, but as already specified above, the deposited DNA sequence associated t species corresponds to P. guibeae, which was later resurrected in Miralles et al. [7] cerning the specimens here identified as P. cf. guibeae, we also did not find any evi of a differentiated sex chromosome system, thus confirming previous observation suggesting that sex chromosomes in this species are probably in an early stage of sification, and mostly pseudo-autosomal.In the P. picta species group, no differen sex chromosomes were observed in P. picta or P. cf. picta, but a ZZ/ZW sex chromo system was reported by Koubová et al. [14] in P. masobe (Figure 4).As previously p out in Koubová et al. [14] and Rovatsos et al. [15], different possible explanations c hypothesized in order to explain the absence/presence of heteromorphic sex chromo pairs and the occurrence of different stages of diversification in the genus Paroedur first hypothesis implies the reversal of differentiated sex chromosomes back to th differentiated state (with a possible sex chromosome turnover), while the secon counts for different diversification rates in distinct clades (see [15]).
Neither hypothesis can be discarded on the basis of the available karyologic molecular data, but we consider the occurrence of homologous sex determinatio tems at different stages of diversification as the most likely and parsimonious scena Paroedura.In fact, sex chromosome pairs usually begin their evolution as highly h Neither hypothesis can be discarded on the basis of the available karyological and molecular data, but we consider the occurrence of homologous sex determination systems at different stages of diversification as the most likely and parsimonious scenario in Paroedura.In fact, sex chromosome pairs usually begin their evolution as highly homologous, pseudoautosomal elements, and their diversification rate (as in other chromosome or nucleotide changes) can be dependent on the occurrence of particular events (e.g., macromutation followed by heterochromatinization and heterochromatin degradation), which are stochastic in nature [31][32][33].As a result, phylogenetically closely related species or even populations may present sex chromosomes that are variable in morphology, heterochromatin content and distribution (see e.g., [34][35][36][37]).
It should also be stressed that the general karyotype structure observed in Paroedura closely resembles that reported for the phylogenetically related geckos of the genera Uroplatus, Matoatoa, Lygodactylus, Ebenavia, Christinus and Phelsuma.In fact, all these gecko genera show a karyotype composed of 2n = 34-42 mostly acrocentric elements, with a tendency towards the formation of biarmed elements via tandem fusions and chromosome inversions (see e.g., [37][38][39][40]).
Considering several characters that are regarded as ancestral karyological features in squamates (e.g., relatively higher total number of chromosomes, ratio of biarmed and acrocentric elements and loci on NORs on the smallest chromosome pairs (see e.g., [39,41,42])), a karyotype of 2n = 38 with all acrocentric elements was recently hypothesized as the ancestral condition in Uroplatus [37] (Figure 4).Starting from a similar karyotype, one tandem fusion would have originated a karyotype of 2n = 36 with one metacentric pair, which is highly represented in Paroedura (see also [13,14]) and can be likely considered as the ancestral condition in the genus (Figure 4).Among the species here studied, this hypothesized ancestral condition would have been conserved in P. picta and P. androyensis, while the different morphologies of the first and second chromosome pair in P. masobe and P. cf. picta, respectively, likely involved two distinct chromosome inversions (Figure 4).In turn, the karyotype of 2n = 34, which appears to be conserved in the P. bastardi group, probably originated from the Paroedura ancestral karyotype by means of a tandem fusion (Figure 4).This evolutionary hypothesis also shows that a comparable pathway of diversification can be observed in the karyotype of different evolutionary lineages of the family Gekkonidae.Indeed, a decrease in the total chromosome number and the progressive formation of biarmed elements via chromosome fusions and inversions is overall one of the most frequently observed karyotype dynamics in squamates (see [42][43][44][45][46][47]). In the genus Paroedura, some chromosome rearrangements should be considered non-homologous, involving different chromosome pairs and potentially driving processes of speciation and lineage diversification.

Conclusions
The intrageneric chromosome variability of the ground geckos of the genus Paroedura involves chromosome number, morphology, and the diversification of sex chromosome systems with female heterogamety (ZZ/ZW).In the P. bastardi species group, chromosomal diversification is apparently mainly linked to the independent differentiation of heterogametic sex chromosome systems, while in two taxa of the P. picta group a different morphology of the second chromosome pair is likely due to an inversion.The general karyotype structure of the genus shares many different features in common with phylogenetically related gecko genera, including the prevalence of acrocentric elements and the progressive formation of biarmed elements by means of chromosome fusions and fissions, which can often be described as non-homologous.Although the genus Paroedura has been the focus of several molecular and cytogenetic studies, our results underline that its taxonomic, genetic and chromosomal diversity should still be considered underestimated.

Figure 1 .
Figure1.Giemsa-stained karyotypes of male (A) and female individuals (B) of P. ibityensis, of male (C) and female individuals (D) of P. rennerae, and female individuals of P. cf. guibeae (E), P. cf. picta (F) and P. picta (G).The boxes show the NOR bearing pair, stained with Giemsa (down) and Ag-NOR staining (up).The scale bar applies to all images.

Figure 1 .
Figure1.Giemsa-stained karyotypes of male (A) and female individuals (B) of P. ibityensis, of male (C) and female individuals (D) of P. rennerae, and female individuals of P. cf. guibeae (E), P. cf. picta (F) and P. picta (G).The boxes show the NOR bearing pair, stained with Giemsa (down) and Ag-NOR staining (up).The scale bar applies to all images.

Animals 2024 ,Figure 4 .
Figure 4. Hypothesized pathways of chromosome diversification in the P. bastardi and P. pic cies groups.

Figure 4 .
Figure 4. Hypothesized pathways of chromosome diversification in the P. bastardi and P. picta species groups.

Table 1 .
Taxonomic attribution, origin and sex of the studied samples of the genus Paroedura.