The genome diversity and karyotype evolution of mammals

The past decade has witnessed an explosion of genome sequencing and mapping in evolutionary diverse species. While full genome sequencing of mammals is rapidly progressing, the ability to assemble and align orthologous whole chromosome regions from more than a few species is still not possible. The intense focus on building of comparative maps for companion (dog and cat), laboratory (mice and rat) and agricultural (cattle, pig, and horse) animals has traditionally been used as a means to understand the underlying basis of disease-related or economically important phenotypes. However, these maps also provide an unprecedented opportunity to use multispecies analysis as a tool for inferring karyotype evolution. Comparative chromosome painting and related techniques are now considered to be the most powerful approaches in comparative genome studies. Homologies can be identified with high accuracy using molecularly defined DNA probes for fluorescence in situ hybridization (FISH) on chromosomes of different species. Chromosome painting data are now available for members of nearly all mammalian orders. In most orders, there are species with rates of chromosome evolution that can be considered as 'default' rates. The number of rearrangements that have become fixed in evolutionary history seems comparatively low, bearing in mind the 180 million years of the mammalian radiation. Comparative chromosome maps record the history of karyotype changes that have occurred during evolution. The aim of this review is to provide an overview of these recent advances in our endeavor to decipher the karyotype evolution of mammals by integrating the published results together with some of our latest unpublished results.


Mammalian Phylogenomics
Modern mammals (Class Mammalia) are divided into three distinct groups ( Figure 1). The subclass Prototheria (monotremes) comprises three species of egg-laying mammals: platypus and two echidna species. The infraclasses Metatheria (marsupials) and Eutheria (placentals) together form the subclass Theria. Over the last decade our understanding of the relationships among eutherian mammals has experienced a virtual revolution. Molecular phylogenomics, new fossils finds and innovative morphological interpretations now group the more than 4600 extant species of eutherians into four major super-ordinal clades: Euarchontoglires (including Primates, Dermoptera, Scandentia, Rodentia, and Lagomorpha), Laurasiatheria (Cetartiodactyla, Perissodactyla, Carnivora, Chiroptera, Pholidota, and Eulipotyphla), Xenarthra, and Afrotheria (Proboscidea, Sirenia, Hyracoidea, Afrosoricida, Tubulidentata, and Macroscelidea) [1]. This modern phylogenetic tree serves as a useful scaffold for combining the various parts of a puzzle in comparative mammalian cytogenetics.

Karyotypes: a global view of the genome
Genes provide instructions to build living organisms and each gene maps to the same chromosome in every cell. Linkage is provided by the co-localization of two or more loci on the same chromosome and the largest linkage group is an entire chromosome. The entire chromosome set of a species is known as a karyotype, which can be thought of as a global map of the nuclear genome.
A seemingly logical consequence of descent from common ancestors is that more closely related species should have more similar chromosomes. However, it is now widely appreciated that species may have phenetically similar karyotypes because they are genomically conservative. Therefore in comparative cytogenetics, phylogenetic relationships should be determined on the basis of the polarity of chromosome differences (derived traits).

Historical development of Comparative Cytogenetics
Mammalian comparative cytogenetics, an indispensable part of phylogenomics, has evolved in a series of steps from a purely descriptive science to a heuristic science of the genomic era. Technical advances have marked the various developmental steps of cytogenetics.

Classical Phase of Cytogenetics
It can be argued that the first step of the Human Genome Project took place when Tjio and Levan in 1956 finally reported the correct diploid number of humans as 2n = 46 [2].
During this phase of cytogenetics, data on the karyotypes of literally hundreds of mammalian species (including information on diploid numbers, relative length and morphology of chromosomes, presence of Bchromosomes) were described ( Figure 2). Diploid numbers (2n) were found to vary from 2n = 6-7 in the Indian muntjac [3] to over 100 in some rodents [4].

Chromosome banding
The second step derived from the invention of C-, G-, R-and other banding techniques and was marked by the Paris Conference (1971) which lead to a standard nomenclature to recognize and classify each human chromosome [5].

G-and R-banding
The most widely used banding methods are G-banding (Giemsa-banding) and R-banding (Reverse-banding). These techniques produce a characteristic pattern of contrasting dark and light transverse bands on the chromosomes. Banding made it possible to identify Figure 1 An evolutionary tree of mammals. The tree depicts historic divergence relationships among the living orders of mammals. The phylogenetic hierarchy is a consensus view of several decades of molecular genetic, morphological and fossil inference (see for example [98,99]. Double rings indicate mammalian supertaxa, numbers indicate the possible time of divergences. homologous chromosomes and construct chromosomal nomenclatures for many species. With banding homologous chromosomes, chromosome segments and rearrangements could be identified. The banded karyotypes of 850 mammalian species were summarized in the Atlas of Mammalian Chromosomes [6]. These basic data present an invaluable resource for the contemporary comparative genomics era, and will assist in selection of new mammalian species for detailed study.

C-banding and heterochromatin
One important source of karyotype variability in mammals is related to heterochromatin. Once the amount of heterochomatin is subtracted from total genome content all mammals have very similar genome sizes.
Species of mammals differ considerably in the heterochromatin content and its location ( Figure 3). Heterochromatin is most often detected using C-banding [7] and early studies using C-banding showed that differences in the fundamental number (i.e., the number of chromosome arms) could be entirely due to the addition of heterochromatic chromosome arms. It is well documented that heterochromatin may consists of different types of repetitive DNA, not all seen with C-banding, and it can vary greatly between karyotypes of even closely related species. The differences of heterochromatin amount among congeneric rodent species may reach 33% of nuclear DNA in Dipodomys species [8], 36% in Peromyscus species [9], 42% in Ammospermophilus [10] and 60% in Thomomys species where C-value (haploid DNA content) ranges between 2.1 and 5.6 pg [11,12]. The red viscacha rat (Tympanoctomys barrerae) has a record C-value among mammals -9.2 pg [13]. Although tetrapoidy was first proposed to be a reason for its high genome size and diploid chromosome number, Svartman et al [14] showed that the high genome size was due to the enormous amplification of heterochromatin. Although one single copy number gene was found to be duplicated in the red viscacha rat genome [15], our data on absence of large genome segment duplications (single paints of most Octodon degu probes) and repetitive DNA hybridization evidence rules against tetraploidy. The study of heterochromatin composition, repeated DNA amount and its distribution on chromosomes of octodontids is absolutely necessary to define exactly what heterochromatin fraction is responsible for the large genomes of the red viscacha rat.
In comparative cytogenetics, chromosome homology between species was proposed on the basis of similarities in banding patterns. Closely related species often had very similar banding pattern and after 40 years of comparing bands it seems safe to generalize that karyotype divergence in most taxonomic groups follows their phylogenetic relationship although there are notable exceptions (see [16] and reviews in [6]).
The conservation of large chromosome segments makes comparison between species possible and worthwhile. On the whole chromosome banding has been a reliable indicator of chromosome homology, i.e. that the chromosome identified on the basis of banding actually carry the same genes. However, this is not always the case especially when phylogenetically distant species or species that have experienced extremely rapid chromosome evolution are compared. Banding after all is still morphology and is not always a foolproof indicator of DNA content.

Comparative molecular cytogenetics
The third step occurred when molecular techniques were incorporated into cytogenetics. These techniques use DNA probes of diverse sizes to compare chromosomes directly at the DNA level. Therefore homology was more confidently compared even between phylogenetically distant species or highly rearranged species (gibbons). Using cladistic analysis rearrangements that have diversified the mammalian karyotype were then more precisely mapped and placed in a phylogenomic perspective. "Comparative chromosomics" -is a new term that was used to define the field of cytogenetics dealing  with recent molecular approaches [17], although "chromosomics" was originally introduced to define the research of chromatin dynamics and morphological changes in interphase chromosome structures [18].
Chromosome painting or Zoo-FISH was the first techniques to have a wide ranging impact [19][20][21][22][23]. With this method the homology of chromosome regions between different species are identified by hybridizing DNA probes of individual, whole chromosomes of one species to metaphase chromosomes of another species ( Figure  4). Comparative chromosome painting allows a rapid and efficient comparison of many species and the distribution of homologous regions makes it possible to track the translocation scenario of chromosomal evolution. When many species covering different mammalian orders are compared, the analysis provides information on trends and rates of chromosomal evolution in different branches.
However, homology is only detected qualitatively, and resolution (about 4 Mb, according to our data) is limited by the size of visualized regions, thus the method does not detect all tiny homologous regions resulted from multiple rearrangements (as between mouse and human). Besides, the method fails to report internal inversions within large segments. Another limitation is that painting across great phylogenetic distance often results in a decreased efficiency. Nevertheless, use of painting probes derived form different species combined with comparative sequencing projects helps to increase the resolution of the method. Chromosome painting sets were made from about 100 vertebrate species (mostly mammals) and the results are summarized in table 1.
In addition to sorting, microdissection of chromosomes and chromosome regions was used to obtain probes for chromosome painting. Impressive results were obtained when a series of microdissection probes covering the total human genome was localized on anthropoid primate chromosomes via multicolor banding (MCB) [24,25]. A limitation of MCB is that it can only be used within a group of closely related species ("phylogenetic" resolution is too low). Spectral karyotyping (SKY) and MFISH -the ratio labeling and simultaneous hybridization of a complete chromosome set have similar drawbacks and have had little application outside of clinical cytogenetics.
All new comparative genomics data including chromosome painting confirmed the high extent of conservation for mammalian chromosomes [23] (Figures 5, 6). Total human chromosomes or their arms can efficiently paint extended chromosome regions in many placentals down to Afrotheria and Xenarthra. Humans are most commonly used as a reference species in chromosome comparisons. Gene localization data on human chromosomes can be extrapolated to the homologous chromosome regions of other species with high reliability. Another surprising feature that facilitates the use of the human genome in comparative studies is that humans are a species with a conserved syntenic chromosome organization that is not so distant from the ancestral condition of all placentals. In Figure 5 we present chromosomal maps of chicken, opossum, and some species of placentals with homologies to human chromosomes and putative mammalian ancestor chromosomes.

Post-genomic time and comparative chromosomics
After the Human Genome Project was completed, researchers focused on evolutionary comparisons of the genome structures of different species. The whole genome of any species can be sequenced completely and repeatedly to obtain a comprehensive, single-nucleotide map. The method makes it possible to compare genomes for any two species regardless of their taxonomic distance. Genome assemblies are available for about 93 fungi; 38 protozoa; 13 plants; more than 40 invertebrates; a few fish, reptiles, and birds; and 38 mammalian species (http://www.genome.gov, http://genome.ucsc. edu, http://www.ncbi.nlm.nih.gov/).
Sequencing efforts provided a host of products that were put to good use in molecular cytogenetics. Fluorescence in situ hybridization (FISH) with DNA clones (BAC and YAC clones, cosmids) allowed the construction of chromosome maps at a resolution of several megabases which could detect relatively small chromosome rearrangements. A resolution of several kilobases can be achieved on interphase chromatin. A limitation is that hybridization efficiencies drop off with increasing phylogenetic distance.  Radiation hybrid (RH) genome mapping is another efficient approach. This method includes the irradiation of cells to disrupt the genome into the desired number of fragments that are subsequently fused with Chinese hamster cells. The resulting somatic cell hybrids contain individual fragments of the genome of interest. Then, 90-100 (sometimes, more) clones covering the total genome are selected, and the sequences of interest are localized on the cloned fragments via the polymerase chain reaction (PCR) or direct DNA-DNA hybridization. To  [61]. Each chromosome is assigned a specific color. These colors are used for mark homologies in idiograms of chromosomes of other species (Figure 5b-5i)  compare the genomes and chromosomes of two species, RHs should be obtained for both of them.

Sex Chromosome Evolution
In contrast to many other taxa, therian mammals and birds are characterized by highly conserved systems of genetic sex determination that lead to special chromosomes, i.e. the sex chromosomes. Although the XX/XY sex chromosome system is the most common among eutherian species, it is not universal. In some species Xautosomal translocations result in the appearance of "additional Y" chromosomes (for example, XX/XY 1 Y 2 Y 3 systems in Black munjac [26,27]). In other species Yautosomal translocations lead to appearance of additional X chromosomes (for example, in some New World primates such as howler monkeys). In this respect rodents again represent a peculiar, derived group, comprising the record number of species with non-classical sex chromosomes such as the wood lemming, the collared lemming, the creep vole, the spinous country rat, the Akodon and the bandicoot rat (reviewed in [28]). One of the most intriguing and enigmatical cases represents the genus of mole voles where Ellobius lutescens has X0/X0 constitution in both sexes ( Figure  2) [29], and -E. alaicus, E. talpinus, E. tancrei have XX/ XX system [30]. Novel methods of genome study have revealed some new interesting data concerning sex chromosome evolution. In monotremes, the most basal mammalian clade, there are multiple sex chromosomes consisting of blocks that are autosomal in therians [31][32][33]. The homologous region to marsupial and eutherian X chromosomes is located on a pair of autosomes in both platypus and echidna [27]. Strikingly there are blocks homologous to the avian Z chromosome, thus presuming a recent origin of therian X [29] and more ancestral mode of avian Z-homologous sex determination as presumed in [34]. This theory is in contrast to comparative painting studies in reptiles and recent lizard genome sequencing project, where most sex chromosomes were found to have no homology with avian Z chromosomes [35,36].
Unfortunately, most current genome sequencing projects ignore Y and W chromosomes. Only the human and chimpanzee Y chromosomes have been sequenced completely [37] and new approaches and studies are necessary to trace the evolution of this essential element of the karyotype in various lineages.

Diploid number polymorphism
Most mammalian species are characterized by a particular chromosome number, but sometimes variation of diploid numbers within a species results from polymorphisms for centric fusions (Robertsonian translocations) involving acrocentric chromosomes. These "Robertsonian fans", were found in many species, including Mus musculus, where all diploid numbers range from 22 to 40 [38]. Another Robertsonian fan was revealed in Sorex araneus with 2n varying from 20 to 33. In both these taxa the number of different karyotypes reaches 60 [39][40][41]. Twenty four different karyotypes were found in Akodon cursor [42] and twenty were found in Gerbillus nigeriae [43].

B-chromosomes
B-chromosomes or dispensable, supernumerary chromosomes were found in certain mammalian species. The number of B-chromosomes (Bs) per cell may vary among different tissues, individuals, and populations. They do not pair and recombine with any of the standard A-chromosomes at meiosis. The Bs occur in about 1.5% of mammalian species, at least two thirds are rodents, mostly from the superfamily Muroideae ( [44], our data). Here we give only two spectacular examples of B-chromosome variation, that were found in the collared lemming Dicrostonyx torquatus, 2N = 40 plus 1 to 42 Bs [45] and in Apodemus peninsulae with 2n = 48 plus 0 to 24 Bs, some of which may be larger than the largest A chromosomes [44]. Figure 2c presents a karyotype of the Siberian Roe deer Capreolus pygargus with eight B-chromosomes [46]. Application of comparative painting has shown that in addition to different heterochromatic blocks [47] B-chromosomes of many mammalian species may contain rather large duplicated segments from autosomes genes and gene segments [48][49][50]. Although transcription and of these genes has not been demonstrated, this finding has led to a change in our view of B-chromosomes and suggests a new role of these elements as harboring genome segment duplications thus giving raw material for appearance of new genes and new combinations of genetic material.

Evolutionary new centromeres
Comparative cytogenetic studies have demonstrated that centromeres are cytogenetic hot spots and that new centromeres occasionally arise. In clinical cytogenetics these events are called "neocentromeres" and "evolutionary new centromeres" or "ENC" in comparative cytogenetics. The first human neocentromere was discovered in 1993 [51]. Later the use of FISH of DNA clones and chromosome painting revealed multiple ENCs in primates [52][53][54][55], perissodactyls [56], rodents [57], marsupials [58] and even birds [59]. ENCs represent a phenomenon that is almost always detected cytogenetically because the centromere is a black hole to most genome sequencing methods.

Reconstructing the Ancestral Mammalian Genome
Comparative painting revealed that particular human chromosomal blocks were often adjacent in a particular phylogenetic array of species. These chromosome associations, often termed evolutionary signatures or landmarks, make it possible to identify the genomic characteristics that are thought to have been present in the common ancestor of the taxons considered. For instance human chromosome signatures 4/8p, 3/21, 14/ 15b, 10p/12a/22a, 16q/19q, 7a/16p, and 12b/22b occur in the genomes of most Boreoeutheria mammals and thus were considered to be characteristic for the genome of their common ancestor. Signature 1/19p and 5/ 21 are found in all Afrotheria and are considered characteristic for this group [60][61][62] (Figure 4). Some workers have suggested that the 1/19 signature, also found in some anteaters (Edentata), was present in the ancestral placental genome [63]. A variant of the ancestral placental genome is shown in Figure 5 [61]. Association HSA1/ 19 was also found in marsupials on Monodelphis chromosome 4 according to sequencing data (http://www. ensembl.org/Monodelphis_domestica), but the associations are not homologous because reciprocal painting shows that the Afrotheria association is 1p/19p while that of the marsupial is 1p36/19q13. Other variants do not include signatures 1/19p and 10p/12a/22, associating the ancestral placental genome mostly with Boreoeutheria [64,65].
Anaylsis of the genome assemblies of mammalian genomes can serve as a test for hypotheses about the content of the ancestral eutherian genome. We expect that the structure of the putative ancestral mammalian genome will be further refined due to new information derived from the genome assemblies of additional mammalian genomes become available. Although purely bioinformatic approaches with a limited number of species [66] has proved unreliable [65], it is clear that a an integration of the two approaches holds promise [67][68][69].
The homologous nature of syntenic associations should be confirmed on a high-resolution basis. Convergent events can be established if the syntenic associations originate from segments derived by different breakpoints. Breakpoints can be established at the cytogenetic level by FISH with cloned DNA such as BACs or at even higher levels of resolution by sequencing. However, breakpoints are often located in duplicated and repeat rich regions of the genome where sequencing is both costly and time consuming. Further, breakpoint reuse may be an additional confounding factor [70]. For example, Robertsonian rearrangements and simple fissions may contribute to homoplasy in cytogenetic analyses.
In spite of these limitations common syntenic associations are still considered as a useful category for phylogenomics. Data on associations of conserved syntenic blocks have been accumulated for all orders of mammals, where each block is identified on the basis of its location on human (HSA) chromosomes. Table 2 lists syntenic associations in a range of animals based on homologies with human chromosomes. It is extremely important to note, that many of ancestral Placentalia chromosomal associations are present not only in eutherians, but also in marsupials and even in birds ( Figure 5). Genome sequencing studies have shown that many ancestral blocks can be found in fish, insects and even in cnidarians [71]. This situation confirms the general rule of high evolutionary genome conservation as first proposed on the basis of chromosome banding up to current comparisons of genome assemblies ( Figures 5, 6).
The most reliable conclusions on the content of ancestral genomes, the pathways and rates of chromosome evolution are made when data is available for the widest possible phylogenetic array of species. Different rates of chromosomal evolution in groups have lead to errors in interpreting phylogenetic relationships. For example, although gibbons are closely related to humans and are included in the Hominoidea, the high number Table 2 The human syntenic associations in genomes of different amniote species of chromosome rearrangements in these taxa makes them phenetically more distant from humans than human are from some species outside the primate order such as cats [72][73][74]. The reasons for high rates of genome reshuffling are far from being clearly understand, still some authors hypothesize that such factors as population structure and the repetitive fraction of DNA content may increase the rate of karyotype evolution [75,76].
In the following paragraphs we will concentrate on particular mammalian orders that were studied by comparative painting which provide particularly informative examples of karyotype evolution.
Canidae A great number of species has been examined by chromosome painting in the order Carnivora, which now, quite naturally, includes pinnipeds (walruses and seals) as a sister group to mustelids. Human chromosome probes detected 30-35 homologous regions on the chromosomes of cats, weasels, lesser panda, pinnipeds, civets, and hyenas; 43-45 regions in the karyotypes of bears and giant panda; and over 70 regions in the canine karyotype. Almost all conserved regions that are characteristic for mammalian ancestral genome and, in particular, for carnivores, are disrupted in the canine genome ( Figures 5, 6B) [77].
It should be noted that the high-quality flow sorted canine chromosome probes [77] proved to be extremely useful for genome mapping. Due to their evolutionary fragmented character, these probes allowed the identification of rearrangements (inversions) within the regions that seem conservative when studied by human chromosome probes ( Figure 6B). As a whole, the use of dog paints has shown that inversions inside of the conservative regions are not frequent. Therefore it is possible that a proportion of the high number of inversions found in many species in mammalian Genome Projects may result from assembly mistakes [78].

Rodentia
Unequal rates of genome evolution have been observed for different mammalian groups; rodents are most remarkable in this respect. The mechanisms that triggered such increased rates of genome reshuffling remain unknown. The order Rodentia comprises more than 40% of all mammalian species. It is the most numerous and evolutionarily diverse taxon of mammals. About one-third of rodent species belong to the superfamily Muroidea (mice, rats, and hamsters). It is muroid rodents that are the champions in the great evolutionary competition, to the shame of other mammalian orders. Comparative reciprocal painting with chromosome probes of mouse and rat showed that the rate of chromosome rearrangements differentiating these extremely close species was tenfold higher than between human and cat, which are rather distant [79]. Yet the most impressive finding was the structure of the mouse genome. After human, mouse Mus musculus is the most thoroughly studied mammal. Early integrative data on mouse chromosome mapping suggested that there were a large number of chromosome rearrangements differentiating the mouse and human genomes [80]. Later, attempts to localize human chromosome probes on mouse chromosomes were, mostly, unsuccessful: the size of many regions homologous in the mouse and human genomes proved lower than the resolution of chromosome painting, confirming that the mouse genome is much more rearranged than that of most other taxa [22]. It is remarkable that the mouse genome includes unusual chromosomes such as chromosome 17, which appears as a "genome dustbin," combining fragments of many chromosomes occurring intact even in other species of the genus Mus ( Figure 5H).
It should be noted that the great number of rearrangements found between humans and the mouse also applies to other Muroidea species, including another well-studied species, the rat, Rattus norvegicus. Thus, in terms of comparative chromosomics, Muroidea appear to have experienced a genomic revolution that sets them apart from the other placental mammals.
Muroid rodents present a particular challenge, considering the high number of species and high rates of chromosome reshuffling. Various techniques are needed to sort out their karyotypic relationships. In addition to flow sorted chromosome paints [81][82][83], a set of chromosome region specific microdissection derived murine probes were used [84]. The hybridization of microdissected murine probes provided a multicolor banding pattern which was particularly useful to identifying new evolutionary breakpoints, previously unrecognized small homologous segments, inversions, and evolutionary new centromeres (discussed above) (Figure 7).
It is important to place on the evolutionary tree the triggering of a mechanism that allowed a considerable increase in the rate of chromosome evolution in rodents. This event took place after Sciuridae (tree squirrels, chipmunks, marmots, and ground squirrels) split from the main lineage of Rodentia. Detailed localization of human chromosome probes on chromosomes of many squirrels and reciprocal painting showed that the squirrel genomes are highly conserved, are similar to the human and ancestral genomes, and have several signatures suggesting a common origin for rodents and lagomorphs [85,86].
The putative karyotype of the rodent ancestor ( Figure  5) is close to the karyotype of placentals and is very distant from that of the Muridae ancestor [81,82,87]. It should be noted that this proposal of rodent ancestral genome organization differs fundamentally from other proposals based on different methods [66]. Bioinformatics approaches up to now are limited because their database is restricted to mouse and rat. The result is a rodent "ancestral genome" intermediate between the human and mouse genomes, which is totally without merit. Only a phylogenetically rich and appropriate array of species may eventually reveal at the bioinformatics level the main regularities of the organization and evolution of mammals and, in particular, rodents.

Perissodactyla
The odd-toed ungulates are a good example to illustrate the potential of chromosome painting for the reconstruction of evolutionary events [88]. This order includes three extant families that have different modes of chromosome evolution. Tapirs and rhinoceroses were found to be extremely conserved and had hardly undergone any rearrangements for millions of years. On the other hand, equids underwent an explosion of karyotype reshuffling accompanied by rapid species divergence. Our data obtained from study of almost all extant representatives of the order (excluding only two Asian rhinoceroses) was subjected to PAUP analysis and resulted in the phylogenetic tree that turned out to be identical to those obtained with sequence analysis data. The phylogeny of equids was particularly easy to reconstruct and non-controversial, probably due to relatively recent fixation of multiple rearrangements.

Cetartiodactyla and chiroptera
The most controversial phylogenies are usually obtained from species, whose divergence occurred long ago and was accompanied by small number of rearrangements. Another problem comes from the appearance of parallelisms or homoplasies. Thus many convergent events were probably characteristic for cetartiodactyls, hampering the reconstruction of non-controversial phylogenetic trees [89]. Convergence and homoplasy was found to be frequent in bats. It was difficult to resolve the phylogeny of the main families in spite of many species involved [90]. Later scrutiny revealed a single association that may reflect the closer relationship of bat families Pteropodidae and Rhinolopoidea [91].

Chromosome painting in resolving superordinal clades
Chromosome-derived characters turned out to be very useful in resolving or supporting some problematic superordinal clades. An example was the support of afrotherian clade at the cytogenetic level. The grouping of Afrotheria was originally based on molecular data [92][1] [93] while paleontological and morphological data did not support the clade. Importantly, independent support came from cytogenetics when two synapomorphic associations, 1/19 and 5/21, were found in all afrotherian species studied [60][62] [94]. Within Afrotheria such clades as Paenungulata (Hyracoidea, Sirenia and Proboscidea) [94,95] and Afroinsectiphillia (aardvark, golden mole, elephant-shrew) [62] were supported by painting data.
Although comparative chromosome painting did not reveal any association uniting all orders of the Laurasiatheria clade (Eulipothypla, Carnivora, Pholidota,  Cetartiodactyla, Perissodactyla, Chiroptera), the order Pinnipedia was placed within Carnivora as sister clade to Mustelidae [97], Cetacea was nested within Artiodactyla [89] and Perissodactyla and Cetartiodactyla were found to be sister clades [63] [88]. All these findings are consistent with most modern phylogenies obtained using molecular data.

Conclusions
The Postgenomic research in mammalian cytogenetics has confirmed the previously established general tendencies of karyotype evolution, brought new data for finalizing phylogenetic trees and allowed a detail analysis of genome evolution in various branches. New molecular approaches led to a precise characterization of breakpoints in evolution and altered our understanding of sex chromosome and B-chromosome evolution.
Studies of mammalian genome evolution are set to take a quantum leap as ever more completely sequenced multiple genomes become available. The previously studied karyotypes characterized from techniques ranging from classical staining and banding to molecular cytogenetic approaches from chromosome paints to cloned DNA will serve as basis for high resolution maps construction for hundreds of mammalian and vertebrate species. A newly proposed Genome 10 K project presumes whole genome sequencing of 10,000 vertebrate species in the near future (G10KCOS 2009), which will provide a foundation for the next generation of postgenomic studies.