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S期小鼠淋巴瘤细胞中化学诱导应激蛋白的差异[32P]标记

Differential [32P]-labeling of chemically induced stress proteins in S-phase mouse lymphoma cells.

作者信息

Pipkin J L, Anson J F, Hinson W G, Burns E R, Casciano D A

机构信息

Department of Health and Human Services, Food and Drug Administration, National Center for Toxicological Research, Jefferson, Arkansas 72079.

出版信息

Appl Theor Electrophor. 1989;1(2):85-94.

PMID:2488593
Abstract

A portion of our research involves the investigation of biomarkers as preclinical indicators of toxic stress. Stemming from this effort, we report three unique proteins that phosphorylate and synthesize during the S-phase of lymphoma cells following chemical insult. Mouse lymphoma cell nuclei were physically sorted (using a fluorescence activated cell sorter) from partitions of the cell cycle and specific nuclear proteins in each partition were examined by gel microelectrophoresis. The changes in [32P]-incorporation by stress proteins (SPs) were examined in each of seven partitions following administration of sodium arsenite. Four SPs [80,000-84,000 relative molecular mass (Mr)], designated 'c','b','x', and 'y', underwent significant alterations in [32P]-labeling and each exhibited varying degrees of differential [32P]-incorporation in partition 3 of G1 phase, all five partitions of S-phase, and partition 1 of G2 phase of the cell cycle. Three other predominantly S-phase SPs (designated S1, S2 and S3) were phosphorylated after sodium arsenite treatment. Stress protein S1 was labeled exclusively in S-phase, while proteins S2 and S3 were labeled only in partition 3 of G1 and S-phase. Stress protein S1 possessed an identical isoelectric point, molecular mass, distribution of polypeptide fragments and immunochemical determinants as S-phase SPs found previously in mouse spleen (X') and mouse liver (LP-S). The identical biochemical characteristics of these three S-phase (SPs), found in diverse tissue types, suggest they are homologous.

摘要

我们的部分研究涉及将生物标志物作为毒性应激的临床前指标进行调查。基于这项工作,我们报告了三种独特的蛋白质,它们在化学损伤后淋巴瘤细胞的S期磷酸化并合成。通过荧光激活细胞分选仪对小鼠淋巴瘤细胞核进行物理分选,从细胞周期的各个部分中分离出来,并通过凝胶微电泳检查每个部分中的特定核蛋白。在给予亚砷酸钠后,对七个部分中的每一个部分中应激蛋白(SPs)的[32P]掺入变化进行了检查。四种SPs[相对分子质量(Mr)为80,000 - 84,000],命名为“c”、“b”、“x”和“y”,在[32P]标记上发生了显著变化,并且在细胞周期的G1期的第3部分、S期的所有五个部分以及G2期的第1部分中均表现出不同程度的差异[32P]掺入。另外三种主要在S期的SPs(命名为S1、S2和S3)在亚砷酸钠处理后被磷酸化。应激蛋白S1仅在S期被标记,而蛋白S2和S3仅在G1期的第3部分和S期被标记。应激蛋白S1具有与先前在小鼠脾脏(X')和小鼠肝脏(LP - S)中发现的S期SPs相同的等电点、分子量、多肽片段分布和免疫化学决定簇。在不同组织类型中发现的这三种S期(SPs)具有相同的生化特征,表明它们是同源的。

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