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菱蛋白和胰岛特异性转录因子-1在胰岛中的表达提示了LIM结构域表位的细胞类型特异性暴露。

Islet expression of Rhombotin and Isl-1 suggests cell type specific exposure of LIM-domain epitopes.

作者信息

Lund K, Petersen J S, Jensen J, Blume N, Edlund T, Thor S, Madsen O D

机构信息

Hagedorn Research Institute, Niels Steensensvej 6, DK2820, Gentofte, Denmark.

出版信息

Endocrine. 1995 Jun;3(6):399-408. doi: 10.1007/BF02935644.

Abstract

The homeodomain protein Isl-1 and the proto-oncogene Rhombotin (a LIM-only protein), share a double zinc-binding LIM domain and have both been implicated in neural and possibly endocrine development. Isl-1 is expressed in all endocrine cell-types of the islet of Langerhans while Rhombotin mRNA expression was reported in rat insulinoma cells. We have cloned and sequenced Rhombotin cDNA from rat insulinoma (99.4% identical to human and mouse sequences) and demonstrate that it is expressed in normal islets, intestinal tissue, and testis, in addition to the brain; but absent in all other organs tested. Rhombotin mRNA is expressed in phenotypically distinct islet tumours (α-, β, and δ-tumours) at levels comparable to that of normal islets. Antisera raised against two distinct epitopes contained within a short synthetic peptide representing part of the N-terminal LIM domain of Rhombotin surprisingly stain α- and δ-cells, respectively, on sections of rat pancreas. Rhombotin is undetectable by immunocytochemistry using LIM-domain antisera on intact monolayer islet tumor cells or transfected fibroblasts while readily detectable when equipped with a FLAG epitope, as detected with FLAG antiserum. In contrast, recombinant FLAG-Rhombotin is efficiently recognised by Western blotting or immunoprecipitation with all LIM-specific antisera. Almost identical results were obtained with LIM-specific versus homeodomain/C-terminal Isl-1 antisera staining α-cell cytoplasm or all islet nuclei, respectively. We conclude that Rhombotin in addition to Isl-1 is expressed in the islet of Langerhans and propose that the differential staining patterns obtained with antisera towards the LIM domains versus flanking epitopes of both proteins reflect (1) cell-specific protein-protein interactions of these domains or, alternatively, (2) islet cell type specific expression of novel homologous LIM domain proteins.

摘要

同源结构域蛋白Isl-1和原癌基因菱框蛋白(一种仅含LIM结构域的蛋白)共享一个双锌结合LIM结构域,并且都与神经发育以及可能的内分泌发育有关。Isl-1在胰岛的所有内分泌细胞类型中均有表达,而菱框蛋白mRNA表达在大鼠胰岛素瘤细胞中被报道。我们已从大鼠胰岛素瘤中克隆并测序了菱框蛋白cDNA(与人和小鼠序列有99.4%的同一性),并证明它除了在脑中表达外,还在正常胰岛、肠道组织和睾丸中表达;但在所检测的所有其他器官中均不存在。菱框蛋白mRNA在表型不同的胰岛肿瘤(α、β和δ肿瘤)中的表达水平与正常胰岛相当。针对代表菱框蛋白N端LIM结构域一部分的短合成肽内两个不同表位产生的抗血清,令人惊讶地分别在大鼠胰腺切片上对α细胞和δ细胞进行染色。使用针对LIM结构域的抗血清在完整的单层胰岛肿瘤细胞或转染的成纤维细胞上进行免疫细胞化学检测时,检测不到菱框蛋白,而当配备FLAG表位时则很容易检测到,用FLAG抗血清检测即可。相比之下,重组FLAG-菱框蛋白能被所有LIM特异性抗血清通过蛋白质印迹法或免疫沉淀法有效识别。用LIM特异性抗血清与同源结构域/C端Isl-1抗血清分别对α细胞胞质或所有胰岛细胞核进行染色,得到了几乎相同的结果。我们得出结论,除了Isl-1外,菱框蛋白也在胰岛中表达,并提出针对这两种蛋白的LIM结构域与侧翼表位的抗血清所获得的不同染色模式反映了(1)这些结构域的细胞特异性蛋白质-蛋白质相互作用,或者(2)新型同源LIM结构域蛋白的胰岛细胞类型特异性表达。

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