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A targeted mutation at the known collagenase cleavage site in mouse type I collagen impairs tissue remodeling.

胶原酶 生物 Ⅰ型胶原 胶原蛋白,I型,α1 突变体 分子生物学 真皮 劈理(地质) 野生型 基因靶向 吸收 细胞生物学 细胞外基质 内分泌学 基因 生物化学 解剖 古生物学 断裂(地质)
作者
Xuedong Liu,Hong Wu,Michael H. Byrne,John J. Jeffrey,Stephen M. Krane,Rudolf Jaenisch
出处
期刊:Journal of Cell Biology [Rockefeller University Press]
卷期号:130 (1): 227-237 被引量:278
标识
DOI:10.1083/jcb.130.1.227
摘要

Degradation of type I collagen, the most abundant collagen, is initiated by collagenase cleavage at a highly conserved site between Gly775 and Ile776 of the alpha 1 (I) chain. Mutations at or around this site render type I collagen resistant to collagenase digestion in vitro. We show here that mice carrying a collagenase-resistant mutant Col1a-1 transgene die late in embryo-genesis, ascribable to overexpression of the transgene, since the same mutation introduced into the endogenous Col1a-1 gene by gene targeting permitted normal development of mutant mice to young adulthood. With increasing age, animals carrying the targeted mutation developed marked fibrosis of the dermis similar to that in human scleroderma. Postpartum involution of the uterus in the mutant mice was also impaired, with persistence of collagenous nodules in the uterine wall. Although type I collagen from the homozygous mutant mice was resistant to cleavage by human or rat fibroblast collagenases at the helical site, only the rat collagenase cleaved collagen trimers at an additional, novel site in the nonhelical N-telopeptide domain. Our results suggest that cleavage by murine collagenase at the N-telopeptide site could account for resorption of type I collagen during embryonic and early adult life. During intense collagen resorption, however, such as in the immediate postpartum uterus and in the dermis later in life, cleavage at the helical site is essential for normal collagen turnover. Thus, type I collagen is degraded by at least two differentially controlled mechanisms involving collagenases with distinct, but overlapping, substrate specificities.

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