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人白细胞介素-12前蛋白亚基的细胞内加工差异:P35信号肽的非典型加工

Disparate intracellular processing of human IL-12 preprotein subunits: atypical processing of the P35 signal peptide.

作者信息

Murphy F J, Hayes M P, Burd P R

机构信息

Division of Cytokine Biology, Center for Biologics Evaluation and Research, Food and Drug Administration, Rockville, MD 20852, USA.

出版信息

J Immunol. 2000 Jan 15;164(2):839-47. doi: 10.4049/jimmunol.164.2.839.

DOI:10.4049/jimmunol.164.2.839
PMID:10623830
Abstract

IL-12 is a heterodimeric cytokine produced by APC that critically regulates cell-mediated immunity. Because of its crucial function during immune responses, IL-12 production is stringently regulated, in part through transcriptional control of its p35 subunit, which requires the differentiative effects of IFN-gamma for expression. To determine whether post-transcriptional aspects of IL-12 production might be regulated, we examined intracellular protein processing of each subunit. We report here that p40 and p35 subunits are processed by disparate pathways. Whereas processing of p40 conforms to the cotranslational model of signal peptide removal concomitant with translocation into the endoplasmic reticulum (ER), processing of p35 does not. Translocation of the p35 preprotein into the ER was not accompanied by cleavage of the signal peptide; rather, removal of the p35 signal peptide occurred via two sequential cleavages. The first cleavage took place within the ER, and the cleavage site localized to the middle of the hydrophobic region of the signal peptide. Although the preprotein was glycosylated upon entry into the ER, its glycosylation status did not affect primary cleavage. Subsequently, the remaining portion of the p35 signal peptide was removed by a second cleavage, possibly involving a metalloprotease, concomitant with additional glycosylation and secretion. Secretion could be inhibited by mutation of the second cleavage site or by inhibition of glycosylation with tunicamycin. In contrast, p40 secretion was not affected by inhibition of glycosylation. Our findings demonstrate that IL-12 subunits are processed by disparate pathways and suggest new modalities for regulation of IL-12 production.

摘要

白细胞介素-12(IL-12)是一种由抗原呈递细胞(APC)产生的异二聚体细胞因子,对细胞介导的免疫起着关键调节作用。由于其在免疫反应中的关键功能,IL-12的产生受到严格调控,部分是通过对其p35亚基的转录控制,而p35亚基的表达需要γ干扰素的分化作用。为了确定IL-12产生的转录后方面是否受到调控,我们研究了每个亚基的细胞内蛋白质加工过程。我们在此报告,p40和p35亚基通过不同途径进行加工。p40的加工符合信号肽去除的共翻译模型,同时转运到内质网(ER)中,而p35的加工则不然。p35前体蛋白转运到内质网中时,信号肽并未裂解;相反,p35信号肽是通过两次连续裂解去除的。第一次裂解发生在内质网内,裂解位点位于信号肽疏水区域的中间。尽管前体蛋白进入内质网后会发生糖基化,但其糖基化状态并不影响初次裂解。随后,p35信号肽的剩余部分通过第二次裂解被去除,可能涉及金属蛋白酶,同时伴随着额外的糖基化和分泌。第二次裂解位点的突变或衣霉素对糖基化的抑制可抑制分泌。相比之下,糖基化抑制并不影响p40的分泌。我们的研究结果表明,IL-12亚基通过不同途径进行加工,并提示了调控IL-12产生的新方式。

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