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利用秀丽隐杆线虫咽部模型研究器官生长过程中细胞外基质重塑的遗传学。

Genetics of extracellular matrix remodeling during organ growth using the Caenorhabditis elegans pharynx model.

机构信息

Department of Cell and Molecular Biology, University of Gothenburg, S-405 30 Gothenburg, Sweden.

出版信息

Genetics. 2010 Nov;186(3):969-82. doi: 10.1534/genetics.110.120519. Epub 2010 Aug 30.

Abstract

The organs of animal embryos are typically covered with an extracellular matrix (ECM) that must be carefully remodeled as these organs enlarge during post-embryonic growth; otherwise, their shape and functions may be compromised. We previously described the twisting of the Caenorhabditis elegans pharynx (here called the Twp phenotype) as a quantitative mutant phenotype that worsens as that organ enlarges during growth. Mutations previously known to cause pharyngeal twist affect membrane proteins with large extracellular domains (DIG-1 and SAX-7), as well as a C. elegans septin (UNC-61). Here we show that two novel alleles of the C. elegans papilin gene, mig-6(et4) and mig-6(sa580), can also cause the Twp phenotype. We also show that overexpression of the ADAMTS protease gene mig-17 can suppress the pharyngeal twist in mig-6 mutants and identify several alleles of other ECM-related genes that can cause or influence the Twp phenotype, including alleles of fibulin (fbl-1), perlecan (unc-52), collagens (cle-1, dpy-7), laminins (lam-1, lam-3), one ADAM protease (sup-17), and one ADAMTS protease (adt-1). The Twp phenotype in C. elegans is easily monitored using light microscopy, is quantitative via measurements of the torsion angle, and reveals that ECM components, metalloproteinases, and ECM attachment molecules are important for this organ to retain its correct shape during post-embryonic growth. The Twp phenotype is therefore a promising experimental system to study ECM remodeling and diseases.

摘要

动物胚胎的器官通常被细胞外基质 (ECM) 覆盖,这些 ECM 必须在胚胎后生长过程中被小心重塑,否则它们的形状和功能可能会受到影响。我们之前描述了秀丽隐杆线虫咽部的扭曲(这里称为 Twp 表型)作为一种随着器官生长而恶化的定量突变表型。先前已知导致咽扭曲的突变会影响具有大细胞外结构域的膜蛋白(DIG-1 和 SAX-7),以及秀丽隐杆线虫 septin(UNC-61)。在这里,我们表明,秀丽隐杆线虫 papilin 基因的两个新等位基因 mig-6(et4)和 mig-6(sa580)也可以引起 Twp 表型。我们还表明,ADAMTS 蛋白酶基因 mig-17 的过表达可以抑制 mig-6 突变体中的咽扭曲,并鉴定出几个与 ECM 相关的基因的等位基因,这些基因可以引起或影响 Twp 表型,包括纤连蛋白 (fbl-1)、多配体聚糖 (unc-52)、胶原蛋白 (cle-1、dpy-7)、层粘连蛋白 (lam-1、lam-3)、一个 ADAM 蛋白酶 (sup-17) 和一个 ADAMTS 蛋白酶 (adt-1) 的等位基因。秀丽隐杆线虫中的 Twp 表型可以通过使用光学显微镜轻松监测,通过测量扭转角度进行定量,并揭示 ECM 成分、金属蛋白酶和 ECM 附着分子对于该器官在胚胎后生长过程中保持正确形状非常重要。因此,Twp 表型是研究 ECM 重塑和疾病的一个很有前途的实验系统。

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