Sex-specific selection on the human X chromosome?

Genes involved in major biological functions, such as reproductive or cognitive functions, are choice targets for natural selection. However, the extent to which these genes are affected by selective pressures remains undefined. The apparent clustering of these genes on sex chromosomes makes this genomic region an attractive model system to study the effects of evolutionary forces. In the present study, we analysed the genetic diversity of a X-linked microsatellite in 1410 X-chromosomes from 10 different human populations. Allelic frequency distributions revealed an unexpected discrepancy between the sexes. By evaluating the different scenarios that could have led to this pattern, we show that sex-specific selection on the tightly linked VCX gene could be the most likely cause of such a distortion.     

Linking X chromosome inactivation to pluripotency: Necessity or fate?

Silencing one X chromosome is essential for the development of female mammals, but the regulation of this process appears to vary between species. In the mouse, which has thus far been the leading model system in the field, X chromosome inactivation (XCI) is tightly coupled to pluripotency and the underlying mechanisms have just begun to be deciphered. However, mechanistic aspects of XCI regulation in other species have yet to be thoroughly investigated. Here we review current knowledge of the developmental regulation of XCI in mice and humans and discuss the extent to which the intimate link between XCI and pluripotency extends beyond rodents.     

Un cas de mosaïcisme avec grand chromosome surnuméraire

Sans résuméRecherches effectuées avec l'appui du Fonds de la Recherche Scientifique Médicale et du Fonds de la Recherche Fondamentale Collective (Belgique).     

Longueur du chromosome Y,intelligence et comportement dans une population de médico-légaux

Summary The Y/F ratio was established in 128 mentally disordered offenders in a maximum security hospital. The 50 Y/F 0.90 subjects were compared with the 78 Y/F<0.90 subjects as regards intelligence and behaviour. With the exception of the highest frequency of intelligence quotients lower than 70 in the criminal patients Y/F 0.90, no statistical correlation exists to support the theory of a relation between a long Y chromosome and the type of psychiatric (psychopathy, psychosis) or criminality diagnosis.

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Mapping through somatic cell hybrids and cDNA probes of protein C to chromosome 2, factor X to chromosome 13, and α1-acid glycoprotein to chromosome 9

Summary The previously unassigned gene coding for the anticoagulatory protein C has been mapped on chromosome 2 using a cDNA probe and genomic blots from a human-hamster somatic cell hybrid panel. The assignments of the genes coding for the coagulation factor X to chromosome 13, and for 1-acid glycoprotein to chromosome 9 have been confirmed using a similar direct approach.     

Génétique moléculaire de la transposition du bras long du chromosome x sur l'y lors de la spéciation humaine

Five cosmidic probes (7 b; 8 j; 22 b; CB 16 and 115 i 1) recognizes site of simple-copy DNA sequence homology between the human X and Y chromosomes. Genomic DNAS restricted with Eco RI from the great apes (Gorilla and Pan) were examined for sequences homologous to these probes, by molecular hybridization studies. Experiments reported here revealed, by genetic dosage with sex, that the great apes have homologous sequences of these five probes on their X chromosomes only. The simplest explanation of these results is that the corresponding sequences were transposed from the X chromosome to the Y chromosome after the human line diverged, like probe pDP 34 for locus DXY S1 (Page et al., 1984).     

Age- and tissue-specific variation of X chromosome inactivation ratios in normal women

The incidence of skewed X-inactivation in normal women is controversial, with up to 10-fold differences being reported by different authors. In order to clarify this issue, we have conducted a survey of the X-inactivation patterns in 270 informative females from various age groups, using the androgen receptor gene/polymerase chain reaction assay. Results obtained by using DNA extracted from blood samples show that the incidence of severe skewing (defined here as ratios > or = 90:10) is relatively common and increases with age (P<0.05), occurring in 7% of women under 25 years of age, and 16% of women over 60. In order to study tissue-specific patterns of X-inactivation, samples of both buccal and urinary epithelia were also obtained from 88 of the females studied. Although there was a significant association of the X-inactivation ratios between each tissue in most individuals, wide variations were apparent in some cases, making accurate extrapolations between tissues impossible. The degree of correlation between each tissue also fell markedly with age. Our data are consistent with the hypothesis that the major factors in the aetiology of skewed X-inactivation are secondary selection processes.     

How does inactivation change timing of replication in the human X chromosome?

Summary The kinetics of replication of the inactive (late replicating) X chromosome (LRX) were studied in karyotypically normal lymphocytes and human amniotic fluid cells. Both cell types were successively pulse labeled with 1-h or 1/2-h thymidine pulses in an otherwise BrdU-substituted S phase after partial synchronization of the cultures at G₁/S. For the first time with this technique, the entire sequence of replication was analyzed for the LRX from the beginning to the end of the S phase, with special reference to mid S (R-band to G-band transition replication). The inactive X is the last chromosome of the metaphase to start replication, with a delay of 1 or 2h, after which time a thymidine pulse results in R-type patterns. In mid S, the inactive X is the first chromosome to switch to G-type replication (without overlapping of both types and without any detectable replication pause). Until the end of S, a thymidine pulse results in G-type patterns. To rule out artifacts that might arise by the synchronization of cultures in these experiments, controls were carried out with BrdU pulses and the BrdU antibody technique without synchronization. In the course of replication, no fundamental difference was seen between the two different cell types examined. In contrast to studies using continuos labeling, this study did not reveal an interindividual difference of replication kinetics in the LRXs of the seven individuals studied; thus it is concluded that the inactive X chromosome shows only one characteristic course of replication.     

Comparaison des séquences de fragments de restriction répétés spécifiques du chromosome Y humain chez le chimpanzé et le gorille

Analysis of the evolutionary conservation and change of the Y human specific Hae III 2.4 kb repeated sequence were studied between man and anthropoïd species after restriction with EcoRI endonuclease. In chimpanzee, blocks of these repeats are absent, the remaining copies being interspersed with other sequences. A close similarity of the restriction patterns of these sequences is found between gorilla and man.     

Molecular characterization of a ring X chromosome in a male with short stature

We report the molecular characterization of a ring X chromosome that was transmitted from a mother to a male who has short stature and minor dysmorphic features. This represents only the second reported ring X chromosome in a male. The ring is derived from breakage within the Xp pseudoautosomal region (PAR) and just proximal to the Xq PAR. The total amount of deleted material is 700-900 kb DNA and includes six known transcribed genes. Interestingly, SHOX, a gene implicated in short stature, is not deleted from the ring chromosome. Possible pathogenetic explanations for the patient's clinical features include insufficient dosage of deleted genes, a position effect on SHOX expression, and cell death during development because of ring chromosome nondisjunction. The findings are also relevant to observations made of "complete" ring chromosomes.     

Un ménage à quatre: the molecular biology of chromosome segregation in meiosis

Sexually reproducing organisms rely on the precise reduction of chromosome number during a specialized cell division called meiosis. Whereas mitosis produces diploid daughter cells from diploid cells, meiosis generates haploid gametes from diploid precursors. The molecular mechanisms controlling chromosome transmission during both divisions have started to be delineated. This review focuses on the four fundamental differences between mitotic and meiotic chromosome segregation that allow the ordered reduction of chromosome number in meiosis: (1) reciprocal recombination and formation of chiasmata between homologous chromosomes, (2) suppression of sister kinetochore biorientation, (3) protection of centromeric cohesion, and (4) inhibition of DNA replication between the two meiotic divisions.     

Existe-il, dans la population générale masculine un risque plus fort de développer des délétions du chromosome Y qui entraîneraient une infertilité?

The role of the Y-chromosome in spermatogenesis remains one of the hottest topics in andrology. Three non overlapping recurrently deleted regions on Yq (AZFa, AZFb, AZFc) have been defined, each of them containing several genes that are candidates for male infertility. The causes and mechanisms leading to microdeletion formation on the Y are largely unknown. Theoretically, it could be possible that some groups of Y-chromosomes (haplogroups) currently distributed in the population could confer a selective advantage/disadvantage towards deletion formation. A precedent in the field is the recent identification of a Y-chromosome haplotype that confers a selective advantage against a translocation of Yp leading to another form of male infertility, the Y+XX-male phenotype. In order to test if selection is acting on Y-chromosome haplotype distribution, we have defined and compared Y-chromosome haplotypes in a group of around 60 individuals with Y microdeletions from North-Western Europe using 10 biallelic Y-markers (SRY-2627, SRY-1532, SRY-8299, 92R7, Tat, YAP, sY81, LLY22g, M9, DYS257). The defined heplotypes were compared to a control normospermic population of the same ethnic/geographic origin (in the framework of the European Biodiversity Project). We evaluatte the relationship between different Y-chromosome backgrounds and microdeletions, and to which extent selection on this chromosome could have influenced fifness of certain individuals/populations. We also discuss the selective forces that are acting on this chromosome and speculate on the mechanisms underlying deletion formation.     

A mitotically stable marker chromosome negative for whole chromosome libraries, centromere probes and chromosome specific telomere regions: a novel class of supernumerary marker chromosome?

A two year-old child presented with mild developmental delay. On karyotype analysis, a supernumerary small marker chromosome (SMC) was found in all cells examined. This SMC was approximately the size of an isochromosome 18p, being symmetrical with a central constriction. C-banding and silver staining were negative and FISH with all chromosome-specific paints, centromere probes and telomere probes showed no hybridization to the SMC; telomere repeat sequences were however present on both arms. Comparative genomic hybridization showed no amplification of any chromosome region. Flow sorting of the SMC and reverse painting onto normal metaphase spreads showed no hybridization to any chromosome, whereas reverse painting onto the patient's own metaphases showed hybridization to the SMC only. This SMC may thus represent either a complex amplicon of different genomic regions, or a multifold amplification of a very small region, with a neocentromere comprising an active kinetochore but no alphoid DNA. Prognostic implications for the proband were difficult to assess due to the absence of reports of similar marker chromosomes in the literature.     

Xéroderma pigmentosum: Huit cas d'évolution différente dans deux familles

Eight cases of xeroderma pigmentosum are described-six in family B. and two in family T. The criteria used in making this diagnosis are indicated. The occurrence of epitheliomas and melanoma was observed. In family B. five of the six patients are alive at time of reporting, their ages varying from 40 to 55 years. In family T. the two affected children died at ages 8 and 14 years. The differential diagnosis between xeroderma pigmentosum and other conditions is briefly discussed.