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在有和没有蛋白酶抑制剂的情况下分离得到的烟草天蛾间隙连接的免疫细胞化学、电泳及免疫印迹分析。

Immunocytochemical, electrophoresis, and immunoblot analysis of Heliothis virescens gap junctions isolated in the presence and absence of protease inhibitors.

作者信息

Ryerse J S

机构信息

Department of Pathology, St. Louis University Health Sciences Center, MO 63104, USA.

出版信息

Cell Tissue Res. 1995 Jul;281(1):179-86. doi: 10.1007/BF00307972.

DOI:10.1007/BF00307972
PMID:7621522
Abstract

Gap junction-enriched fractions were prepared from larvae of the tobacco budworm Heliothis virescens using the NaOH procedure in the presence or absence of protease inhibitors and were analyzed by SDS-PAGE immunoblotting and EM immunocytochemistry. Protease inhibitor fractions contained a 48-kDa protein in addition to the approximately 10 proteins in fractions with and without inhibitors. Three polyclonal antibodies were used as probes for gap junction plaques and proteins: R16, against an approximately 40-kDa candidate gap junction protein from Drosophila melanogaster; R17, against the 40-kDa candidate gap junction protein from H. virescens; and R18AP, an affinity purified antibody against a consensus sequence of N-terminal amino acids 2-21 of the H. virescens 40-kDa protein. R16, R17, and R18AP stain the 40- and 48-kDa proteins, R16 and R18AP stain a 64-kDa protein, and R16 stains an approximately 30-kDa protein in the absence of inhibitors. Inclusion of protease inhibitors had no effect on gap junction ultrastructure. R16 and R17 label gap junction plaques in crude membrane and NaOH fractions, whereas R18AP exhibits only a low level of reactivity with gap junctions in crude membrane fractions and none with gap junctions in NaOH fractions. The results show that the 30-, 40-, 48- and 64-kDa proteins are immunologically related and are associated with gap junctions in H. virescens, the N-terminus of the 40-kDa protein is relatively inaccessible or easily lost, and the 48-kDa protein is protease-sensitive.

摘要

采用NaOH法,在有或无蛋白酶抑制剂的情况下,从烟草天蛾幼虫中制备富含间隙连接的组分,并通过SDS-PAGE免疫印迹和EM免疫细胞化学进行分析。除了有或无抑制剂的组分中大约10种蛋白质外,蛋白酶抑制剂组分还含有一种48 kDa的蛋白质。三种多克隆抗体用作间隙连接斑块和蛋白质的探针:R16,针对来自黑腹果蝇的一种约40 kDa的候选间隙连接蛋白;R17,针对来自烟草天蛾的40 kDa候选间隙连接蛋白;以及R18AP,一种针对烟草天蛾40 kDa蛋白N端氨基酸2-21共有序列的亲和纯化抗体。R16、R17和R18AP可对40 kDa和48 kDa的蛋白质进行染色,R16和R18AP可对一种64 kDa的蛋白质进行染色,在没有抑制剂的情况下,R16可对一种约30 kDa的蛋白质进行染色。加入蛋白酶抑制剂对间隙连接的超微结构没有影响。R16和R17标记粗膜和NaOH组分中的间隙连接斑块,而R18AP与粗膜组分中的间隙连接仅表现出低水平的反应性,与NaOH组分中的间隙连接则无反应。结果表明,30 kDa、40 kDa、48 kDa和64 kDa的蛋白质在免疫上相关,且与烟草天蛾的间隙连接相关,40 kDa蛋白质的N端相对难以接近或容易丢失,48 kDa蛋白质对蛋白酶敏感。

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1
Immunocytochemical, electrophoresis, and immunoblot analysis of Heliothis virescens gap junctions isolated in the presence and absence of protease inhibitors.在有和没有蛋白酶抑制剂的情况下分离得到的烟草天蛾间隙连接的免疫细胞化学、电泳及免疫印迹分析。
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