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人中性粒细胞胶原酶的纯化及单特异性抗血清的制备。

Purification of human neutrophil collagenase and production of a monospecific antiserum.

作者信息

Christner P, Damato D, Reinhart M, Abrams W

出版信息

Biochemistry. 1982 Nov 9;21(23):6005-11. doi: 10.1021/bi00266a043.

DOI:10.1021/bi00266a043
PMID:6295451
Abstract

Although there is good evidence for the presence of human neutrophil (PMN) collagenase, only moderate purification has been reported. The probable explanation for this fact is that most assays used to specifically measure collagenase activity are not reliable if high levels of several different proteases are also present in the assay mixture. The PMN granule is just such a concentrated mixture. Therefore, polyacrylamide gel electrophoresis was used to identify and quantitate the alpha 1 3/4 and alpha 2 3/4 cleavage products diagnostic for mammalian collagenase. White cells (85% PMN's) were lysed in 0.34 M sucrose and granules were obtained. The granules were lysed by sonication, and the lysate was chromatographed on a Sephadex G-200 column followed by a Trasylol-Sepharose 4B column. This procedure resulted in a 1350-fold purification and a yield of 75 micrograms of enzyme/unit of blood. The collagenase was inhibited by ethylene glycol bis(beta-aminoethyl ether)-N,N,N',N'-tetraacetic acid but not by sulfhydryl or serine protease inhibitors. The preparation was free of elastase, which has been shown to cleave type III collagen into alpha 1 3/4 and alpha 1 1/4 pieces. The pI of collagenase was shown to be 4.7 by isoelectric focusing, and the enzyme lost activity below a pH of 6.5 if collagen was absent. Antiserum was produced by 100-micrograms injections of the purified collagenase into rabbits. Titers were measured by the enzyme-linked immunosorbent assay. For determination of the specificity, collagenase and PMN extract were isoelectrically focused and blotted onto nitrocellulose. The antibody recognized only one band of protein in the PMN extract, which comigrated with the purified collagenase.

摘要

尽管有充分证据表明人中性粒细胞(PMN)胶原酶的存在,但仅报道了中度纯化。这一事实的可能解释是,如果测定混合物中还存在几种不同的高水平蛋白酶,那么大多数用于特异性测量胶原酶活性的测定方法都不可靠。PMN颗粒就是这样一种浓缩混合物。因此,使用聚丙烯酰胺凝胶电泳来鉴定和定量对哺乳动物胶原酶具有诊断意义的α1 3/4和α2 3/4裂解产物。将白细胞(85%为PMN)在0.34 M蔗糖中裂解,获得颗粒。通过超声处理使颗粒裂解,裂解物先在Sephadex G - 200柱上进行层析,然后在抑肽酶 - Sepharose 4B柱上进行层析。该程序实现了1350倍的纯化,每单位血液产生75微克酶。胶原酶被乙二醇双(β - 氨基乙醚)- N,N,N',N'-四乙酸抑制,但不受巯基或丝氨酸蛋白酶抑制剂抑制。该制剂不含弹性蛋白酶,弹性蛋白酶已被证明可将III型胶原裂解为α1 3/4和α1 1/4片段。通过等电聚焦显示胶原酶的pI为4.7,如果没有胶原,该酶在pH值低于6.5时会失去活性。通过向兔子注射100微克纯化的胶原酶产生抗血清。通过酶联免疫吸附测定法测量效价。为了确定特异性,将胶原酶和PMN提取物进行等电聚焦并印迹到硝酸纤维素膜上。抗体在PMN提取物中仅识别一条与纯化胶原酶共迁移的蛋白带。

相似文献

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Purification of human neutrophil collagenase and production of a monospecific antiserum.人中性粒细胞胶原酶的纯化及单特异性抗血清的制备。
Biochemistry. 1982 Nov 9;21(23):6005-11. doi: 10.1021/bi00266a043.
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Systematic separation and purification of elastase, gelatinase (matrix metalloproteinase 9), and collagenase (matrix metalloproteinase 8) from polymorphonuclear leukocytes in dialyzers previously used by patients with renal failure.从肾衰竭患者先前使用过的透析器中的多形核白细胞中系统分离和纯化弹性蛋白酶、明胶酶(基质金属蛋白酶9)和胶原酶(基质金属蛋白酶8)。
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引用本文的文献

1
Heterogeneity among human collagenases demonstrated by monoclonal antibody that selectively recognizes and inhibits human neutrophil collagenase.单克隆抗体证明人胶原酶之间存在异质性,该单克隆抗体可选择性识别并抑制人中性粒细胞胶原酶。
J Exp Med. 1984 May 1;159(5):1455-63. doi: 10.1084/jem.159.5.1455.
2
Granulocyte collagenase and cathepsin B in patients with cancer of digestive organs.消化器官癌症患者体内的粒细胞胶原酶和组织蛋白酶B
Gastroenterol Jpn. 1984 Dec;19(6):537-42. doi: 10.1007/BF02793867.
3
Human fibroblast collagenase: glycosylation and tissue-specific levels of enzyme synthesis.
人成纤维细胞胶原酶:糖基化与酶合成的组织特异性水平
Proc Natl Acad Sci U S A. 1986 Jun;83(11):3756-60. doi: 10.1073/pnas.83.11.3756.
4
Hypochlorous acid (HOCl) activation of neutrophil collagenase requires cathepsin G.中性粒细胞胶原酶的次氯酸(HOCl)激活需要组织蛋白酶G。
Agents Actions. 1989 Jun;27(3-4):481-4. doi: 10.1007/BF01972858.
5
Activation of neutrophil collagenase by cathepsin G.组织蛋白酶G对中性粒细胞胶原酶的激活作用。
Inflammation. 1989 Jun;13(3):245-58. doi: 10.1007/BF00914392.