A study of chromosome association in hybrids between diploid species of Festuca

Hybrids between the two diploid species Festuca donax and F. drymeja had regular chromosome association, forming 7 bivalents at metaphase I. However, when the two species were crossed with a third species F. scariosa, the hybrids involving F. drymeja showed greater desynapsis than those with F. donax. When the F₁ hybrid F. donax × F. drymeja was crossed with F. scariosa, the trispecific progeny could be grouped into three classes according to the degree of desynapsis recorded. Abnormalities associated with the fusion of pollen mother cells, which produced highly polyploid cells, were also observed in the trispecific hybrids. Failure of chromosomal pairing and the occurrence of syncytes is attributed to genotypic interactions.     

The genetics of self-incompatibility inOenothera rhombipetala

Pollen tubes were grown under controlled temperatures in stigmas and styles which had been cut from the flowers at the point of juncture of the style with the ovary. At constant temperatures the tubes compatible with the styles grew rapidly at uniform rates. They showed accelerated growth with increase in temperature within the range 10°–30°C. Growth of incompatible tubes was irregular and slow and was neither measurably accelerated nor depressed within this range of temperatures. Routine tests for compatibility were conducted at 27°C; at this temperature compatible tubes grew through the entire length of the styles (ca. 58 mm) in 9 hours. Much of the incompatible pollen failed to germinate; that which did, grew to a maximum length ofca. 2 mm inca. 4 hours. The incompatible tubes did not even enter the styles but remained confined to the stigmas. ThreeS alleles were involved and conformed in their behavior to the gametophytic system of incompatibility. Colchicine-induced tetraploid derivatives of these plants showed no increase in compatibility.     

Genetic regulation of chromosome behaviour in interspecific hybrids of Drosophila

Summary When crossing Drosophila virilis females with D. littoralis males, the elimination of D. littoralis sixth chromosome (microchromosomes) was often observed. The absence of the sixth chromosome of D. littoralis was revealed when studying F₁ hybrids, because of the mosaic expression of the recessive gene gl, located in the sixth chromosome of D. virilis. In the reciprocal cross the elimination of the sixth chromosome of D. littoralis did not take place (Sokolov 1959).Genetic analysis enabled the authors to conclude that the observed maternal effect on mitosis is controlled by recessive genes located on the second and fourth chromosome of D. virilis. The genes located on the second chromosome, differ from those on the fourth chromosome both in temperature sensitivity and in the time and/ or the mechanism controlling the mitotic behaviour of the chromosomes.By means of back-crosses a new stock was established where all chromosomes except the sixth belonged to D. virilis. The sixth pair (microchromosomes) in this line was represented by one D. virilis and one D. littoralis chromosome. It was shown that the sixth chromosome of D. littoralis might be eliminated or undergo non-disjunction in D. virilis germline but the frequency of such atypical behaviour was very low (about 2 %). Low temperature treatment was not effective for increasing the frequency of either elimination or non-disjunction of the D. littoralis sixth chromosome in D. virilis germ-line.     

Quantitative study of organelle nucleoids during the second pollen grain mitosis inOenothera biennis

Summary The behavior of organelle nucleoids in the generative cell was examined at the second (pollen grain) mitosis by epifluorescence microscopy after staining with 4,6-diamidino-2-phenylindole (DAPI) inOenothera biennis. TheO. biennis generative cell contained a large number of organelle nucleoids distributed randomly in the cytoplasm before mitosis. The epifluorescence images of the nucleoids could be classified distinctly into two groups which corresponded to plastid nucleoids (pt-nucleoids) and mitochondrial nucleoids (mt-nucleoids). Discrimination between pt- and mt-nucleoids was carried out with the aid of DNA immunogold electron microscopy. At metaphase, both pt- and mt-nucleoids migrated to the pole regions of the generative cell. After mitosis, organelle nucleoids in both of the sperm cells scattered in the cytoplasm again. A quantitative examination of pt-nucleoids on 202 pairs of sperm cells showed that the leading sperm cell (Svn) contained 0–39 pt-nucleoids (19.0 ± 7.4) and the trailing sperm cell (Sua) contained 0–40 pt-nucleoids (15.4 ± 6.5). For mt-nucleoids, examination of 28 pairs of sperm cells showed that Svn contained 5–32 mt-nucleoids (14.5 ± 6.8) and Sua contained 6–30 mt-nucleoids (13.4 ±7.5). These results showed that (1) the number of organelle nucleoids per sperm cell varied considerably in the cells studied; (2) quantitative difference in pt- and mt-nucleoids between Svn and Sua could occur in some gametophytes studied; but (3) it was unlikely that there was any pre-differentiational cytoplasm localization and essential sperm heteromorphy with respect to organelle nucleoid content in the gametophyte population.     

Physical mapping of human chromosome 17 using fragment-containing microcell hybrids

Hybrid cell lines were generated by microcell-mediated transfer of human chromosome 17 into rat recipient cells. The genotypes of 36 such lines were analyzed using a set of human chromosome 17-derived sequences to probe the structural integrity of the chromosome. Four classes of hybrids were obtained: clones with an apparently intact chromosome 17, clones containing large fragments of the chromosome including both the centromere and the selected marker, clones containing only the selected marker and flanking sequences, and clones containing two 17-derived fragments--the pericentric region plus the region of the selected marker. Data from these hybrids were used in conjunction with published regional localization information to obtain a provisional linear map of the chromosome. Results of this analysis are compared to the gene maps predicted from recent linkage studies and from other somatic cell hybrid experiments.     

Assignment of the gene for lactic dehydrogenase A to mouse chromosome 7 using mouse-human hybrids

We have studied somatic cell hybrids between either mouse peritoneal macrophages or spleen cells and HT-1080-6TG human fibrosarcoma cells for the expression of mouse lactic dehydrogenase A (LDH-A). The hybrids were also studied for the expression of mouse glucose phosphate isomerase (GPI-1), the gene for which has been assigned to chromosome 7. Concordant segregation of the expression of mouse GPI-1 and LDH-1 was observed in 61 independent hybrid clones. These results indicate that the gene coding for LDH-A is located on mouse chromosome 7.     

A chromosome study in multiple sclerosis

Summary Chromosome studies of 30 patients with multiple sclerosis and 30 controls have been made. The results show that there is no significant increase in the frequency of structural aberrations in the multiple sclerosis patients. It is suggested that previously reported differences may have been due to technical factors, the nature of which is discussed.

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Zusammenfassung Bei 30 Patienten mit multipler Sklerose und 30 Kontrollen wurden die Chromosomen untersucht. Es fand sich bei den Patienten kein signifikanter Anstieg in der Häufigkeit struktureller Aberrationen. Vielleicht wurden früher mitgeteilte Unterschiede durch technische Faktoren, die im einzelnen diskutiert werden, vorgetäuscht.