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猪血小板中性粒细胞趋化蛋白的分子克隆与特性分析

Molecular cloning and characterisation of a neutrophil chemotactic protein from porcine platelets.

作者信息

Power C A, Proudfoot A E, Magnenat E, Bacon K B, Wells T N

机构信息

Glaxo Institute for Molecular Biology, Geneva, Switzerland.

出版信息

Eur J Biochem. 1994 Apr 15;221(2):713-9. doi: 10.1111/j.1432-1033.1994.tb18784.x.

DOI:10.1111/j.1432-1033.1994.tb18784.x
PMID:7513641
Abstract

In our search for novel chemoattractant factors, we have purified a heparin-binding protein from porcine platelets which is a potent chemoattractant for human neutrophils. The protein has 80 amino acids and a molecular mass of 8597.5Da as measured by electrospray mass spectrometry. It has been characterised by amino acid sequencing and shown to have highest identity to members of the human platelet basic-protein-family. Its N-terminal sequence is intermediate in length between the human connective-tissue-activating polypeptide III (CTAP-III) and neutrophil-activating polypeptide-2 (NAP-2). The porcine NAP-2/CTAP-III shows the classic CXC cysteine spacing found towards the N-terminus in the chemokine alpha family and contains the ELR motif which has been shown to be essential for neutrophil chemotaxis. We have isolated mRNA from porcine platelets and constructed a cDNA library containing 1.0 x 10(6) independent clones. Using probes based on the protein sequence we have isolated a full length-clone for this gene, with an open reading frame containing 119 amino acids. Despite overall similarity between the human and porcine proteins, the N-terminal region is almost completely different between the two species, with only two identical amino acids. The proteolytic cleavage sites required for processing of human platelet basic protein are completely missing in the porcine homologue, implying a different processing pathway or mechanism. The porcine protein is capable of agonizing certain effects of both NAP-2 and CTAP-III when incubated with human cells indicating that the same porcine protein may be involved in both processes.

摘要

在寻找新型趋化因子的过程中,我们从猪血小板中纯化出一种肝素结合蛋白,它是人类中性粒细胞的强效趋化剂。通过电喷雾质谱法测定,该蛋白有80个氨基酸,分子量为8597.5Da。已通过氨基酸测序对其进行了表征,结果显示它与人类血小板碱性蛋白家族成员具有最高的同源性。其N端序列的长度介于人类结缔组织激活多肽III(CTAP-III)和中性粒细胞激活多肽2(NAP-2)之间。猪NAP-2/CTAP-III在趋化因子α家族的N端显示出典型的CXC半胱氨酸间隔,并且含有ELR基序,该基序已被证明对中性粒细胞趋化作用至关重要。我们从猪血小板中分离出mRNA,并构建了一个包含1.0×10⁶个独立克隆的cDNA文库。利用基于该蛋白序列的探针,我们分离出了该基因的全长克隆,其开放阅读框包含119个氨基酸。尽管人类和猪的蛋白总体相似,但两种物种的N端区域几乎完全不同,只有两个相同的氨基酸。猪同源物中完全没有人类血小板碱性蛋白加工所需的蛋白水解切割位点,这意味着其加工途径或机制不同。当与人类细胞一起孵育时,猪蛋白能够引发NAP-2和CTAP-III的某些效应,这表明相同的猪蛋白可能参与了这两个过程。

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Molecular cloning and characterisation of a neutrophil chemotactic protein from porcine platelets.猪血小板中性粒细胞趋化蛋白的分子克隆与特性分析
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