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P-4和RNKP-7,在活化大鼠淋巴细胞中表达的新型颗粒酶样丝氨酸蛋白酶。

P-4 and RNKP-7, new granzyme-like serine proteases expressed in activated rat lymphocytes.

作者信息

Ewoldt G R, Smyth M J, Darcy P K, Harris J L, Craik C S, Horowitz B, Woodard S L, Powers J C, Hudig D

机构信息

Department of Microbiology, School of Medicine, University of Nevada, Reno 89557, USA.

出版信息

J Immunol. 1997 May 15;158(10):4574-83.

PMID:9144469
Abstract

Serine proteases (granzymes) in killer lymphocytes are required for lymphocyte cytotoxic granules to lyse target cells. Herein we report the development of a 3-step PCR cloning technique to amplify novel granzyme genes and two new rat granzymes are described. Degenerate oligonucleotide primers were designed based on sequence motifs selectively expressed in granzymes. These motifs flank "delta" regions that are unique for each granzyme. Total RNA of RNK-16 cells or activated splenocytes was amplified by reverse transcriptase-PCR to obtain cDNA fragments of several new granzymes. Gene-specific primers based on these delta regions were then used for 3'-RACE to obtain clones with the 3' gene ends. Reverse (antisense) delta-based or active site serine primers were used with a granzyme 5'-UTR primer to obtain clones extending to the 5' ends. Using this technique, two new cDNAs, RNKP-4 and RNKP-7, which encode granzymes of 248 and 241 amino acids, respectively, were cloned from activated lymphocytes. RNKP-4 is likely the rat equivalent of mouse granzyme C. RNKP-7 is most closely related to granzymes F and G. Modeling of the predicted proteins suggests large/polar P1 (Gln/Asn) specificity for RNKP-4 and large/hydrophobic P1 (e.g., Phe) specificity for RNKP-7. These specific protease activities were found in cytotoxic RNK-16 lymphocyte granules indicating that the two new genes may be translated and stored as active granzymes.

摘要

杀伤淋巴细胞中的丝氨酸蛋白酶(颗粒酶)是淋巴细胞细胞毒性颗粒裂解靶细胞所必需的。在此我们报告了一种三步PCR克隆技术的开发,用于扩增新的颗粒酶基因,并描述了两种新的大鼠颗粒酶。基于在颗粒酶中选择性表达的序列基序设计了简并寡核苷酸引物。这些基序位于每个颗粒酶特有的“δ”区域两侧。通过逆转录PCR扩增RNK-16细胞或活化脾细胞的总RNA,以获得几种新颗粒酶的cDNA片段。然后基于这些δ区域的基因特异性引物用于3'-RACE,以获得具有3'基因末端的克隆。使用基于δ的反向(反义)引物或活性位点丝氨酸引物与颗粒酶5'-UTR引物一起获得延伸至5'末端的克隆。使用该技术,从活化的淋巴细胞中克隆了两个新的cDNA,RNKP-4和RNKP-7,它们分别编码248和241个氨基酸的颗粒酶。RNKP-4可能相当于大鼠的小鼠颗粒酶C。RNKP-7与颗粒酶F和G关系最为密切。对预测蛋白质的建模表明,RNKP-4具有大/极性P1(Gln/Asn)特异性,RNKP-7具有大/疏水性P1(例如Phe)特异性。在细胞毒性RNK-16淋巴细胞颗粒中发现了这些特定的蛋白酶活性,表明这两个新基因可能被翻译并作为活性颗粒酶储存。

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J Immunol. 1997 May 15;158(10):4574-83.
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