The structural and functional analyses of heterochromatin are essential to understanding how heterochromatic genes are regulated and how centromeric chromatin is formed. Because the repetitive nature of heterochromatin hampers its genome analysis, new approaches need to be developed. Here, we describe how, in double mutants for Su(var)3-9 and SuUR genes encoding two structural proteins of heterochromatin, new banded heterochromatic segments appear in all polytene chromosomes due to the strong suppression of under-replication in pericentric regions. FISH on salivary gland polytene chromosomes from these double mutant larvae allows high resolution of heterochromatin mapping. In addition, immunostaining experiments with a set of antibodies against euchromatic and heterochromatic proteins reveal their unusual combinations in the newly appeared segments: binding patterns for HP1 and HP2 are coincident, but both are distinct from H3diMetK9 and H4triMetK20. In several regions, partial overlapping staining is observed for the proteins characteristic of active chromatin RNA Pol II, H3triMetK4, Z4, and JIL1, the boundary protein BEAF, and the heterochromatin-enriched proteins HP1, HP2, and SU(VAR)3-7. The exact cytological position of the centromere of chromosome 3 was visualized on salivary gland polytene chromosomes by using the centromeric dodeca satellite and the centromeric protein CID. This region is enriched in H3diMetK9 and H4triMetK20 but is devoid of other proteins analyzed.

译文

:异染色质的结构和功能分析对于了解异色基因如何调控以及着丝粒染色质如何形成至关重要。由于异染色质的重复性质妨碍了其基因组分析,因此需要开发新的方法。在这里,我们描述了如何在Su(var)3-9和SuUR基因的双突变体中编码异染色质的两个结构蛋白,新条带化的异色片段由于强烈抑制外周中心区域的复制不足而在所有多烯染色体中出现。这些双突变幼虫在唾液腺多态染色体上的FISH可以实现高分辨率的异染色质定位。此外,使用针对常染色体和异源蛋白质的抗体的免疫染色实验在新出现的片段中揭示了它们的不寻常组合:HP1和HP2的结合模式是重合的,但两者均不同于H3diMetK9和H4triMetK20。在几个区域中,观察到活性染色质RNA Pol II,H3triMetK4,Z4和JIL1,边界蛋白BEAF和富含异染色质的蛋白HP1,HP2和SU(VAR)3-7的蛋白具有部分重叠染色。 。通过使用着丝粒十二指肠卫星和着丝粒蛋白CID,在唾液腺多烯染色体上可以看到3号染色体着丝粒的确切细胞学位置。该区域富含H3diMetK9和H4triMetK20,但没有其他被分析的蛋白质。

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