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利用针对不均一核糖核蛋白的抗体对多线染色体进行分布研究。

Distribution studies on polytene chromosomes using antibodies directed against hnRNP.

作者信息

Christensen M E, LeStourgeon W M, Jamrich M, Howard G C, Serunian L A, Silver L M, Elgin S C

出版信息

J Cell Biol. 1981 Jul;90(1):18-24. doi: 10.1083/jcb.90.1.18.

Abstract

The distribution of nuclear ribonucleoprotein (hnRNP) particles in Drosophila polytene chromosomes has been investigated using anti-B-36 serum as a probe. The use of polytene chromosomes allows resolution at the level of the chromomere, and provides the opportunity to look for both positive and negative correlations with transcriptional activity. The antiserum was obtained using the nuclear protein B-36 from Physarum polycephalum as the immunogen. It has been shown to precipitate hnRNP particles from HeLa cells through a cross-reaction with the major 32,000- and 34,000-dalton hnRNP particle proteins. The antiserum cross-reacts with a Drosophila nuclear protein of approximately 34,000 daltons. By indirect immunofluorescence, we observed that the antiserum reacts preferentially with transcriptionally active loci of the polytene chromosomes, whereas loci previously or subsequently active do not show significant fluorescence. The overall pattern of fluorescence is very similar to that generated with anti-RNA polymerase B serum. The correlation of fluorescence and transcriptional activity observed suggests that the anti-B-36 serum is recognizing hnRNP proteins which have combined with nascent RNA molecules at the sites of transcription.

摘要

利用抗B - 36血清作为探针,研究了核核糖核蛋白(hnRNP)颗粒在果蝇多线染色体中的分布。多线染色体的使用使得在染色粒水平上能够分辨,并提供了寻找与转录活性正相关和负相关的机会。该抗血清是用多头绒泡菌的核蛋白B - 36作为免疫原获得的。已证明它能通过与主要的32000道尔顿和34000道尔顿的hnRNP颗粒蛋白发生交叉反应,从HeLa细胞中沉淀出hnRNP颗粒。该抗血清与一种约34000道尔顿的果蝇核蛋白发生交叉反应。通过间接免疫荧光,我们观察到该抗血清优先与多线染色体的转录活性位点发生反应,而先前或随后活跃的位点则没有明显的荧光。荧光的总体模式与用抗RNA聚合酶B血清产生的模式非常相似。观察到的荧光与转录活性之间的相关性表明,抗B - 36血清识别的是在转录位点与新生RNA分子结合的hnRNP蛋白。

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