Extent and rate of chromosome segregation in two intraspecific mouse cell hybrids: A9 x diploid foetal erythrocyte and A9 x B82.

Patterns of chromosome segregation were studied in 2 different intraspecific mouse cell hybrids: (1) A9 x B82, formed by fusing 2 cell lines of heteroploid fibroblasts, and (2) UWE, originating from the fusion of A9 cells with euploid foetal erythrocytes. Detailed analyses of Giemsa (G)-banded chromosomes and chromosome arms of both parental and hybrid cells were made for each hybrid type, in order to determine the specificity of the losses and to assess the influence of ploidy and cell differentiation. Unlike the A9 x B82 hybrids, which revealed a significant chromosome loss under selective tissue culture pressures only after 9 months, the UWE hybrids showed a sharp reduction in the total chromosome number during the initial 2 months under similar pressures. However, with no additional cloning, UWE remained karyotypically stable after that time. This rapid chromosomal segregation in UWE hybrids may be caused by properties of the parental foetal erythrocytes. In UWE cells, the majority of the chromosome arms were retained or duplicated. Less than a quarter of the total number of chromosome arms were segregated or lost, and these were all chromosome arms with abnormal mouse G-banding patterns, present only in the heteroploid A9 parental cells. In two of the four A9 x B82 hybrid lines, there was marked segregation of chromosome arms whose banding patterns were identical to those of wild type mouse telocentric chromosomes. For both types of intraspecific cell hybrids, two thirds or more of the chromosome arms had banding patterns which were the same as those of the wild type genome.