Freddo Andrew M, Shoffner Suzanne K, Shao Yue, Taniguchi Kenichiro, Grosse Ann S, Guysinger Margaux N, Wang Sha, Rudraraju Shiva, Margolis Benjamin, Garikipati Krishna, Schnell Santiago, Gumucio Deborah L
Department of Cell and Developmental Biology, University of Michigan Medical School, Ann Arbor, MI 48109, USA.
Integr Biol (Camb). 2016 Sep 12;8(9):918-28. doi: 10.1039/c6ib00046k. Epub 2016 Aug 1.
Efficient digestion and absorption of nutrients by the intestine requires a very large apical surface area, a feature that is enhanced by the presence of villi, fingerlike epithelial projections that extend into the lumen. Prior to villus formation, the epithelium is a thick pseudostratified layer. In mice, villus formation begins at embryonic day (E)14.5, when clusters of mesenchymal cells form just beneath the thick epithelium. At this time, analysis of the flat lumenal surface reveals a regular pattern of short apical membrane invaginations that form in regions of the epithelium that lie in between the mesenchymal clusters. Apical invaginations begin in the proximal intestine and spread distally, deepening with time. Interestingly, mitotically rounded cells are frequently associated with these invaginations. These mitotic cells are located at the tips of the invaginating membrane (internalized within the epithelium), rather than adjacent to the apical surface. Further investigation of epithelial changes during membrane invagination reveals that epithelial cells located between mesenchymal clusters experience a circumferential compression, as epithelial cells above each cluster shorten and widen. Using a computational model, we examined whether such forces are sufficient to cause apical invaginations. Simulations and in vivo data reveal that proper apical membrane invagination involves intraepithelial compressive forces, mitotic cell rounding in the compressed regions and apico-basal contraction of the dividing cell. Together, these data establish a new model that explains how signaling events intersect with tissue forces to pattern apical membrane invaginations that define the villus boundaries.
肠道对营养物质的高效消化和吸收需要非常大的顶端表面积,绒毛的存在增强了这一特征,绒毛是延伸到肠腔的指状上皮突起。在绒毛形成之前,上皮是一层厚厚的假复层。在小鼠中,绒毛形成始于胚胎第14.5天(E14.5),此时间充质细胞簇在厚上皮下方形成。此时,对平坦的管腔表面进行分析,发现在间充质细胞簇之间的上皮区域形成了规则的短顶端膜内陷模式。顶端内陷始于近端肠道并向远端扩散,随着时间的推移而加深。有趣的是,有丝分裂变圆的细胞经常与这些内陷相关。这些有丝分裂细胞位于内陷膜的尖端(内化在上皮内),而不是靠近顶端表面。对膜内陷期间上皮变化的进一步研究表明,位于间充质细胞簇之间的上皮细胞受到周向压缩,因为每个细胞簇上方的上皮细胞缩短并变宽。我们使用计算模型研究了这种力是否足以导致顶端内陷。模拟和体内数据表明,适当的顶端膜内陷涉及上皮内压缩力、压缩区域内的有丝分裂细胞变圆以及分裂细胞的顶-基收缩。这些数据共同建立了一个新模型,解释了信号事件如何与组织力相互作用,以形成界定绒毛边界的顶端膜内陷模式。