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体内微管是可用的β-微管蛋白同种型的共聚物:使用合成肽抗原引发的多克隆抗体对六种脊椎动物β-微管蛋白同种型进行定位。

In vivo microtubules are copolymers of available beta-tubulin isotypes: localization of each of six vertebrate beta-tubulin isotypes using polyclonal antibodies elicited by synthetic peptide antigens.

作者信息

Lopata M A, Cleveland D W

机构信息

Department of Biological Chemistry, Johns Hopkins University School of Medicine, Baltimore, Maryland 21205.

出版信息

J Cell Biol. 1987 Oct;105(4):1707-20. doi: 10.1083/jcb.105.4.1707.

Abstract

beta-Tubulin is encoded in the genomes of higher animals by a small multigene family comprising approximately seven functional genes. These genes produce a family of closely related, but distinct polypeptide isotypes that are distinguished principally by sequences within the approximately 15 carboxy-terminal amino acid residues. By immunizing rabbits with chemically synthesized peptides corresponding to these variable domain sequences, we have now prepared polyclonal antibodies specific for each of six distinct isotypes. Specificity of each antiserum has been demonstrated unambiguously by antibody binding to bacterially produced, cloned proteins representing each isotype and by the inhibition of such binding by preincubation of each antiserum only with the immunizing peptide and not with heterologous peptides. Protein blotting of known amounts of cloned, isotypically pure polypeptides has permitted accurate quantitative measurement of the amount of each beta-tubulin isotype present in the soluble and polymer forms in various cells, but has not revealed a bias for preferential assembly of any isotype. Localization of each isotype in three different cell types using indirect immunofluorescence has demonstrated that in vivo each class of microtubules distinguishable by light microscopy is assembled as copolymers of all isotypes expressed in a single cell.

摘要

β-微管蛋白在高等动物基因组中由一个小的多基因家族编码,该家族包含大约七个功能基因。这些基因产生一系列密切相关但又不同的多肽同工型,主要通过大约15个羧基末端氨基酸残基内的序列来区分。通过用与这些可变结构域序列相对应的化学合成肽免疫兔子,我们现在制备了针对六种不同同工型中每一种的多克隆抗体。每种抗血清的特异性已通过抗体与代表每种同工型的细菌产生的克隆蛋白结合以及通过仅用免疫肽而非异源肽预孵育每种抗血清来抑制这种结合而得到明确证明。对已知量的克隆的、同型纯多肽进行蛋白质印迹分析,可以准确地定量测量各种细胞中可溶性和聚合物形式的每种β-微管蛋白同工型的含量,但尚未发现对任何同工型优先组装的偏好。使用间接免疫荧光法在三种不同细胞类型中定位每种同工型已证明,在体内,通过光学显微镜可区分的每类微管都是由单个细胞中表达的所有同工型的共聚物组装而成。

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