小鼠膜型-1-基质金属蛋白酶（MT-1-MMP）的克隆及其在肾后肾发育过程中对基质金属蛋白酶-2（MMP-2）及其抑制剂的调控

Cloning of murine membrane-type-1-matrix metalloproteinase (MT-1-MMP) and its metanephric developmental regulation with respect to MMP-2 and its inhibitor.

作者信息

Ota K, Stetler-Stevenson W G, Yang Q, Kumar A, Wada J, Kashihara N, Wallner E I, Kanwar Y S

机构信息

Department of Pathology and Medicine, Northwestern University Medical School, Chicago, Illinois, USA.

出版信息

Kidney Int. 1998 Jul;54(1):131-42. doi: 10.1046/j.1523-1755.1998.00XXX.x.

DOI:10.1046/j.1523-1755.1998.00XXX.x

PMID:9648071

Abstract

BACKGROUND

Extracellular matrix macromolecules regulate morphogenesis of embryonic organs, and are developmentally regulated. Their expression and turnover is regulated by matrix metalloproteinases (MMPs). Recently, an epithelial cell "membrane" associated metalloproteinase (MT-1-MMP) has been identified that acts as an activator of a "secreted" MMP-2, and is produced by mesenchymal fibroblasts. The activity of MMP-2 is inhibited by a "soluble" tissue inhibitor of MMP-2, TIMP-2. The role of MT-1-MMP in renal development is unknown.

METHODS

MT-1-MMP was cloned from embryonic mouse kidney cDNA library, and its spatio-temporal distribution during development in the context of MMP-2 and tissue inhibitor of metalloproteinase-2 (TIMP-2) was studied.

RESULTS

The cloned MT-1-MMP exhibited approximately 86% nucleotide sequence homology with human MT-1-MMP, and had a catalytic domain and a zinc binding site preceded by a RRKR furin recognition motif. A approximately 4.5 Kb MT-1-MMP mRNA transcript was detected, and its expression was developmentally regulated. A parallel developmental regulation of MMP-2 mRNA expression was also observed. TIMP-2 expression was also developmentally regulated, but lagged behind MT-1-MMP and MMP-2. By in situ hybridization, MT-1-MMP mRNA was seen to be confined to ureteric bud epithelia, and was absent in the mesenchyme, while MMP-2 was confined to the mesenchyme. MT-1-MMP protein expression was seen on ureteric bud epithelia, induced mesenchyme and nascent nephrons, and it was highest during mid gestation. Similar spatio-temporal expressions of MMP-2 and TIMP-2 proteins were observed.

CONCLUSIONS

mRNAs of MT-MMP-1 and MMP-2 are expressed in the respective epithelial and mesenchymal compartments, while their proteins are co-expressed in the epithelia suggest that MT-1-MMP and MMP-2, in conjunction with TIMP-2, may be involved in paracrine/juxtacrine epithelial:mesenchymal interactions during metanephrogenesis.

摘要

背景

细胞外基质大分子调节胚胎器官的形态发生，且受发育调控。它们的表达和更新由基质金属蛋白酶（MMPs）调节。最近，已鉴定出一种与上皮细胞“膜”相关的金属蛋白酶（MT-1-MMP），它作为“分泌型”MMP-2的激活剂，由间充质成纤维细胞产生。MMP-2的活性受到“可溶性”MMP-2组织抑制剂TIMP-2的抑制。MT-1-MMP在肾脏发育中的作用尚不清楚。

方法

从胚胎小鼠肾脏cDNA文库中克隆MT-1-MMP，并研究其在发育过程中与MMP-2和金属蛋白酶-2组织抑制剂（TIMP-2）相关的时空分布。

结果

克隆的MT-1-MMP与人类MT-1-MMP的核苷酸序列同源性约为86%，具有一个催化结构域和一个锌结合位点，其前面有一个RRKR弗林蛋白酶识别基序。检测到一个约4.5kb的MT-1-MMP mRNA转录本，其表达受发育调控。还观察到MMP-2 mRNA表达的平行发育调控。TIMP-2表达也受发育调控，但滞后于MT-1-MMP和MMP-2。通过原位杂交，MT-1-MMP mRNA局限于输尿管芽上皮，间充质中不存在，而MMP-2局限于间充质。MT-1-MMP蛋白表达见于输尿管芽上皮、诱导的间充质和新生肾单位，在妊娠中期最高。观察到MMP-2和TIMP-2蛋白类似的时空表达。