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74-kD细胞质动力蛋白亚基与鞭毛动力蛋白多肽的同源性表明其具有细胞内靶向功能。

Homology of the 74-kD cytoplasmic dynein subunit with a flagellar dynein polypeptide suggests an intracellular targeting function.

作者信息

Paschal B M, Mikami A, Pfister K K, Vallee R B

机构信息

Cell Biology Group, Worcester Foundation for Experimental Biology, Shrewsbury, Massachusetts 01545.

出版信息

J Cell Biol. 1992 Sep;118(5):1133-43. doi: 10.1083/jcb.118.5.1133.

Abstract

In previous work we found cytoplasmic dynein to be a complex of two catalytic heavy chains and at least seven co-purifying polypeptides of unknown function. The most prominent of these is a 74-kD electrophoretic species which can be resolved as two to three bands by SDS-PAGE. We have now selected a series of overlapping rat brain cDNAs encoding the 74-kD species. The deduced sequence of a full-length cDNA predicts a 72,753 D polypeptide which includes the amino acid sequences of nine peptides determined by NH2-terminal microsequencing. PCR performed on first strand rat brain cDNA together with the sequence of a partially matching tryptic peptide indicated the existence of at least three isoforms of the 74-kD cytoplasmic dynein subunit. Comparison with known sequences revealed that the carboxyl-terminal half of the polypeptide is 26.4% identical and 47.7% similar to the product of the Chlamydomonas ODA6 gene, a 70-kD intermediate chain of flagellar outer arm dynein. Immunoblot analysis with a monoclonal antibody to the 74-kD species indicated a widespread tissue distribution, as expected for a cytoplasmic dynein subunit. Nonetheless, the antibody recognized a 67-kD species in ram sperm flagella and pig tracheal cilia, supporting the existence of distinct but related cytoplasmic and axonemal polypeptides in mammals. In view of evidence for a role for the ODA6 gene product in anchoring flagellar dynein to the A subfiber microtubule in the axoneme, we predict an analogous role for the 74-kD polypeptide, perhaps in mediating the interaction of cytoplasmic dynein with membranous organelles and kinetochores.

摘要

在先前的工作中,我们发现胞质动力蛋白是由两条催化重链和至少七条功能未知的共纯化多肽组成的复合物。其中最显著的是一种74-kD的电泳条带,通过SDS-PAGE可解析为两到三条带。我们现已筛选出一系列编码该74-kD条带的重叠大鼠脑cDNA。全长cDNA的推导序列预测出一个72,753 D的多肽,其中包括通过氨基末端微测序确定的九个肽段的氨基酸序列。对大鼠脑cDNA第一链进行的PCR以及部分匹配的胰蛋白酶肽段序列表明,74-kD胞质动力蛋白亚基至少存在三种同工型。与已知序列比较发现,该多肽的羧基末端一半与衣藻ODA6基因的产物有26.4%的同一性和47.7%的相似性,ODA6基因产物是鞭毛外臂动力蛋白的一种70-kD中间链。用针对74-kD条带的单克隆抗体进行的免疫印迹分析表明,其在组织中广泛分布,这与胞质动力蛋白亚基的预期情况相符。尽管如此,该抗体在公羊精子鞭毛和猪气管纤毛中识别出一种67-kD的条带,这支持了哺乳动物中存在不同但相关的胞质和轴丝多肽。鉴于有证据表明ODA6基因产物在将鞭毛动力蛋白锚定到轴丝中的A亚纤维微管上起作用,我们预测74-kD多肽也有类似作用,可能在介导胞质动力蛋白与膜性细胞器和动粒的相互作用中发挥作用。

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