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腺苷脱氨酶缺陷型人淋巴母细胞系中的免疫反应性蛋白。

Immunoreactive protein in adenosine deaminase deficient human lymphoblast cell lines.

作者信息

Wiginton D A, Hutton J J

出版信息

J Biol Chem. 1982 Mar 25;257(6):3211-7.

PMID:6977542
Abstract

Adenosine deaminase (adenosine aminohydrolase, EC 3.5.4.4) was examined in human lymphoblast cell lines from normal and adenosine deaminase-deficient individuals as well as individuals heterozygous for adenosine deaminase deficiency. Adenosine deaminase activity was determined by a specific enzymatic assay and compared to immunoreactive adenosine deaminase protein (or cross-reacting material) determined by radioimmunoassay, in order to investigate mutations affecting adenosine deaminase. Two different antisera, raised in goat and rabbit against human adenosine deaminase, had different sensitivities and apparent specificities when used for radioimmunoassay. Rabbit antisera provided the most sensitive assay of normal enzyme, whereas goat antiserum provided the most sensitive assay for detection of mutant proteins. A wide range of values for the ratio of immunoreactive protein to activity was observed for the adenosine deaminase deficient cell lines, ranging from near normal to 23 times normal. The cell lines with high ratios appear to contain large amounts of catalytically defective or inactive protein. The amount of mutant protein detected by radioimmunoassay in the deficient cell lines depends upon the antiserum utilized, making as much as a 50-fold difference. The heterozygous lines contain approximately half of the normal amounts of immunoreactive protein and activity, and thus have a normal ratio of the two. Two cell lines partially deficient in adenosine deaminase appear to contain large amounts of an unstable adenosine deaminase protein with partially impaired activity. Immunoreactive protein was visualized in extracts from several cell lines, after electrophoresis and transfer to activated paper, by labeling with immunological probes and autoradiography.

摘要

对来自正常个体、腺苷脱氨酶缺乏个体以及腺苷脱氨酶缺乏杂合子个体的人淋巴母细胞系中的腺苷脱氨酶(腺苷氨基水解酶,EC 3.5.4.4)进行了检测。通过特定的酶促测定法测定腺苷脱氨酶活性,并与通过放射免疫测定法测定的免疫反应性腺苷脱氨酶蛋白(或交叉反应物质)进行比较,以研究影响腺苷脱氨酶的突变。用山羊和兔子制备的两种不同抗人腺苷脱氨酶血清在用于放射免疫测定时具有不同的敏感性和表观特异性。兔抗血清对正常酶的检测最为敏感,而山羊抗血清对突变蛋白的检测最为敏感。在腺苷脱氨酶缺乏的细胞系中观察到免疫反应性蛋白与活性的比值范围很广,从接近正常到正常的23倍。比值高的细胞系似乎含有大量催化缺陷或无活性的蛋白。在缺乏的细胞系中通过放射免疫测定法检测到的突变蛋白量取决于所使用的抗血清,相差可达50倍。杂合子细胞系含有约一半正常量的免疫反应性蛋白和活性,因此两者的比值正常。两个腺苷脱氨酶部分缺乏的细胞系似乎含有大量不稳定的腺苷脱氨酶蛋白,其活性部分受损。通过用免疫探针标记和放射自显影,在电泳并转移到活性纸上后,可以在几个细胞系的提取物中观察到免疫反应性蛋白。

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