Robbins J R, McGuire P G, Wehrle-Haller B, Rogers S L
Department of Cell Biology and Physiology, University of New Mexico School of Medicine, 149 Basic Medical Sciences Building, Albuquerque, New Mexico, 87131, USA.
Dev Biol. 1999 Aug 15;212(2):255-63. doi: 10.1006/dbio.1999.9373.
Platelet-derived growth factors (PDGF) regulate cell proliferation, survival, morphology, and migration, as well as deposition and turnover of the extracellular matrix. Important roles for the A form of PDGF (PDGF-A) during connective tissue morphogenesis have been highlighted by the murine Patch mutation, which includes a deletion of the alpha subunit of the PDGF receptor. Homozygous (Ph/Ph) embryos exhibit multiple connective tissue defects including cleft face (involving the first branchial arch and frontonasal processes), incomplete heart septation, and heart valve abnormalities before they die in utero. Analyses of the cell biology underlying the defects in Ph/Ph embryos have revealed a deficit in a matrix metalloproteinase (MMP-2) and one of its activators (MT-MMP) that are likely to be involved in cell migration and tissue remodeling, two processes necessary for normal cardiac and craniofacial development. Morphogenesis of these structures requires infiltration of ectomesenchymal precursors and their subsequent deposition and remodeling of extracellular matrix components. First branchial arch and heart tissue from E10.5 embryos were examined by gelatin zymography and RT-PCR in order to characterize the expression of MMPs in these tissues. Of the MMPs examined, only MMP-2 and one of its activators, MT-MMP, were expressed in the first arch and heart at this stage of development. Tissues from Ph/Ph embryos exhibited a significant decrease in both MMP-2 and MT-MMP compared to tissues from normal embryos of the same developmental stage. In order to assess whether this decrease affects the motile activity of mesenchymal cells, cell migration from Ph/Ph branchial arch explants was compared to migration from normal arch tissue and found to be significantly less. In addition, the migratory ability of branchial arch cells from normal explants could be reduced in a similar manner using a specific MMP inhibitor. Although it is still unclear whether the MMP-2 reduction is a direct result of the absence of response of Ph/Ph cells to PDGF-A treatment of normal branchial arch cells in vitro with recombinant PDGF-AA significantly upregulated MMP-2 protein. Together, these results suggest that PDGF-A regulates MMP-2 expression and activation during normal development and that faulty proteinase expression may be at least partially responsible for the developmental defects exhibited by Ph/Ph embryos.
血小板衍生生长因子(PDGF)可调节细胞增殖、存活、形态、迁移以及细胞外基质的沉积和更新。小鼠的Patch突变突出了PDGF的A形式(PDGF-A)在结缔组织形态发生过程中的重要作用,该突变包括PDGF受体α亚基的缺失。纯合子(Ph/Ph)胚胎在子宫内死亡前表现出多种结缔组织缺陷,包括腭裂(涉及第一鳃弓和额鼻突)、心脏间隔不完全以及心脏瓣膜异常。对Ph/Ph胚胎缺陷背后的细胞生物学分析表明,一种基质金属蛋白酶(MMP-2)及其激活剂之一(MT-MMP)存在缺陷,这可能与细胞迁移和组织重塑有关,而这两个过程是正常心脏和颅面发育所必需的。这些结构的形态发生需要外间充质前体的浸润及其随后对细胞外基质成分的沉积和重塑。通过明胶酶谱法和RT-PCR检测了E10.5胚胎的第一鳃弓和心脏组织,以表征这些组织中MMPs的表达。在所检测的MMPs中,只有MMP-2及其激活剂之一MT-MMP在发育的这个阶段在第一鳃弓和心脏中表达。与相同发育阶段正常胚胎的组织相比,Ph/Ph胚胎的组织中MMP-2和MT-MMP均显著降低。为了评估这种降低是否影响间充质细胞的运动活性,将Ph/Ph鳃弓外植体的细胞迁移与正常鳃弓组织的迁移进行了比较,发现前者明显较少。此外,使用特异性MMP抑制剂可以以类似的方式降低正常外植体鳃弓细胞的迁移能力。虽然尚不清楚MMP-2的降低是否是Ph/Ph细胞对PDGF-A无反应的直接结果,但用重组PDGF-AA体外处理正常鳃弓细胞可显著上调MMP-2蛋白。总之,这些结果表明,PDGF-A在正常发育过程中调节MMP-2的表达和激活,蛋白酶表达异常可能至少部分导致了Ph/Ph胚胎出现的发育缺陷。
