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骨外植体在培养过程中以无活性的酶原形式释放胶原酶。

The release of collagenase as an inactive proenzyme by bone explants in culture.

作者信息

Vaes G

出版信息

Biochem J. 1972 Jan;126(2):275-89. doi: 10.1042/bj1260275.

Abstract
  1. A latent collagenase, activated only by limited proteolysis, was found in culture media of mouse bone explants. It could be activated by trypsin or, less efficiently, by chymo-trypsin. Skin explants also released latent collagenase. 2. Bone collagenase attacks native collagen at about neutral pH when it is in solution, in reconstituted fibrils or in insoluble fibres, producing two fragments representing 75 and 25% of the molecule. It requires calcium and is inhibited by EDTA, cysteine or serum. 3. Latent collagenase is not activated by trypsin-activated collagenase but by a distinct unidentified thermolabile agent present in a latent trypsin-activatable state in the culture media, or by purified liver lysosomes between pH5.5 and pH7.4. Trypsin activation decreases the molecular weight of latent collagenase from 105000 to 84000 as determined by gel filtration. 5. The latency of collagenase is unlikely to be due to an enzyme-inhibitor complex. Although some culture media contain a collagenase inhibitor, its presence is not constant and its molecular weight (at least 120000) is not compatible with the decrease in molecular weight accompanying activation; also combinations of collagenase with inhibitor are not reactivated by trypsin. Moreover, the latency remains after gel filtration, or treatment by high dilution, exposure to pH values between 2.5 and 10, or high ionic strength, urea or detergent. 6. It is proposed that latent collagenase represents an inactive precursor of the enzyme, a ;procollagenase', and that the extracellular activity of collagenase is controlled by another protease that activates procollagenase by a limited proteolysis of its molecule.
摘要
  1. 在小鼠骨外植体的培养基中发现了一种仅通过有限的蛋白水解作用激活的潜在胶原酶。它可被胰蛋白酶激活,或被胰凝乳蛋白酶激活,但效率较低。皮肤外植体也能释放潜在胶原酶。2. 骨胶原酶在中性pH左右时,能攻击处于溶液状态、重组原纤维状态或不溶性纤维状态的天然胶原,产生两个片段,分别占分子的75%和25%。它需要钙,且受乙二胺四乙酸(EDTA)、半胱氨酸或血清抑制。3. 潜在胶原酶不会被胰蛋白酶激活的胶原酶激活,而是被培养基中以潜在的可被胰蛋白酶激活状态存在的一种独特的未鉴定的热不稳定因子激活,或被pH5.5至pH7.4之间的纯化肝溶酶体激活。通过凝胶过滤测定,胰蛋白酶激活会使潜在胶原酶的分子量从105000降至84000。5. 胶原酶的潜伏性不太可能是由于酶 - 抑制剂复合物。虽然一些培养基含有胶原酶抑制剂,但其存在并不恒定,且其分子量(至少120000)与激活时伴随的分子量降低不相符;此外,胶原酶与抑制剂的组合不会被胰蛋白酶重新激活。而且,经过凝胶过滤、高倍稀释处理、暴露于pH值在2.5至10之间、高离子强度、尿素或去污剂处理后,潜伏性仍然存在。6. 有人提出,潜在胶原酶代表该酶的无活性前体,即“前胶原酶”,并且胶原酶的细胞外活性由另一种蛋白酶控制,该蛋白酶通过对前胶原酶分子进行有限的蛋白水解作用来激活它。

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