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使用痘苗病毒载体研究人类疾病中的蛋白质加工。家族性自主神经功能异常患者培养成纤维细胞中正常神经生长因子的加工与分泌。

Use of vaccinia virus vectors to study protein processing in human disease. Normal nerve growth factor processing and secretion in cultured fibroblasts from patients with familial dysautonomia.

作者信息

Edwards R H, Rutter W J

机构信息

Hormone Research Institute, University of California, San Francisco 94143.

出版信息

J Clin Invest. 1988 Jul;82(1):44-7. doi: 10.1172/JCI113599.

Abstract

Familial dysautonomia is a hereditary disorder that affects autonomic and sensory neurons. Nerve growth factor (NGF) is required for the normal development of sympathetic and sensory neurons and it has been postulated that an abnormality involving NGF may be responsible for familial dysautonomia. Previous studies have shown that the beta-NGF gene is not linked to the disease. However, NGF appears to be abnormal by immunochemical assays; the putative altered form of NGF could result from a disturbance in the processing pathway. To study the processing of the 35-kD glycosylated NGF precursor and the secretion of NGF in familial dysautonomia, we have employed a recombinant vaccinia virus vector to express high levels of NGF mRNA in primary fibroblast cultures from patients with the disorder; the processing pathway was then studied directly. Cells from several unrelated patients all produce the same 35-kD NGF precursor, process this normally to NGF within the cell, and release NGF into the medium. There are no differences in the ability of cells from patients and from unaffected relatives to process and secrete NGF. The use of similar recombinant vaccinia virus vectors to express proteins at high level in primary cell lines should facilitate the detection of posttranslational processing defects in a variety of human disorders.

摘要

家族性自主神经功能异常是一种影响自主神经和感觉神经元的遗传性疾病。神经生长因子(NGF)是交感神经和感觉神经元正常发育所必需的,据推测,涉及NGF的异常可能是家族性自主神经功能异常的病因。以往的研究表明,β-NGF基因与该疾病并无关联。然而,免疫化学分析显示NGF似乎存在异常;推测NGF的改变形式可能是加工途径紊乱所致。为了研究家族性自主神经功能异常中35-kD糖基化NGF前体的加工过程以及NGF的分泌情况,我们利用重组痘苗病毒载体在患有该疾病患者的原代成纤维细胞培养物中高水平表达NGF mRNA;随后直接研究加工途径。来自几位不相关患者的细胞均产生相同的35-kD NGF前体,在细胞内将其正常加工为NGF,并将NGF释放到培养基中。患者细胞与未受影响亲属的细胞在加工和分泌NGF的能力上并无差异。利用类似的重组痘苗病毒载体在原代细胞系中高水平表达蛋白质,应有助于检测各种人类疾病中的翻译后加工缺陷。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/d3ac/303474/235d51a7efeb/jcinvest00079-0054-a.jpg

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