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DNA修复甲基转移酶在人类细胞中的细胞内定位及功能

Intracellular localization and function of DNA repair methyltransferase in human cells.

作者信息

Ishibashi T, Nakabeppu Y, Kawate H, Sakumi K, Hayakawa H, Sekiguchi M

机构信息

Department of Biochemistry, Kyushu University, Fukuoka, Japan.

出版信息

Mutat Res. 1994 Nov;315(3):199-212. doi: 10.1016/0921-8777(94)90032-9.

Abstract

An antibody preparation specific for human O6-methylguanine-DNA methyltransferase (EC 2.1.1.63) was obtained by immunoaffinity purification on two types of affinity columns with the purified human and mouse methyltransferase proteins as ligands. The antibodies were used in Western blotting analysis of fractionated cell extracts. More than 90% of the methyltransferase protein was recovered in the cytoplasmic fractions with both human HeLa S3 cells and MR-M cells, the latter overproducing the enzyme 36 times as much as the former. Cytoplasmic localization of the methyltransferase in HeLa S3 cells was further confirmed by in situ immunostaining. By Western blotting analysis of fractionated cell extracts from HeLa S3 cells treated with alkylating agents, we found that amounts of the enzyme decreased more rapidly in the nuclear fraction than in the cytoplasmic fraction, and recovery of the enzyme level in the cytoplasmic fraction was slower than that in the other. These results suggest that the methyltransferase protein is degraded in the nucleus after it commits the repair reaction and that the cytoplasmic enzyme is transported into the nucleus as the nuclear methyltransferase is used up in this manner.

摘要

通过在两种以纯化的人源和鼠源甲基转移酶蛋白为配体的亲和柱上进行免疫亲和纯化,获得了对人O6-甲基鸟嘌呤-DNA甲基转移酶(EC 2.1.1.63)具有特异性的抗体制剂。这些抗体用于分级分离的细胞提取物的蛋白质印迹分析。在人HeLa S3细胞和MR-M细胞的细胞质组分中均回收了超过90%的甲基转移酶蛋白,后者产生该酶的量是前者的36倍。原位免疫染色进一步证实了HeLa S3细胞中甲基转移酶的细胞质定位。通过对用烷化剂处理的HeLa S3细胞分级分离的细胞提取物进行蛋白质印迹分析,我们发现该酶在细胞核组分中的减少速度比在细胞质组分中更快,并且细胞质组分中酶水平的恢复比另一个组分更慢。这些结果表明,甲基转移酶蛋白在完成修复反应后在细胞核中被降解,并且随着细胞核中的甲基转移酶以这种方式被耗尽,细胞质中的酶被转运到细胞核中。

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