Simon T C, Roth K A, Gordon J I
Department of Molecular Biology, Washington University School of Medicine, St. Louis, Missouri 63110.
J Biol Chem. 1993 Aug 25;268(24):18345-58.
Axial pattern formation is sustained in the mammalian gut epithelium despite rapid and continuous renewal of its four principal cell lineages. The mouse and rat liver fatty acid-binding protein (L-FABP) genes (Fabpl) represent an excellent model for understanding the mechanisms that determine differentiation-dependent, cell lineage-specific, and distinct regional patterns of expression along the crypt-to-villus and duodenal-to-ileal axes of the gut, as well as within the liver acinus. We have used transgenic mice to map cis-acting elements in rat Fabpl that control these patterns of gene expression. Seven transgenes were analyzed, representing sequential deletions of the 5'-nontranscribed domain of Fabpl linked to the human growth hormone (hGH) gene beginning at its nucleotide +3 (L-FABP/hGH+3). Several pedigrees of mice containing each one of the L-FABP/hGH+3 transgenes were examined at the end of their 8th and 20th weeks of postnatal life using immunocytochemical and RNA hybridization analyses. A remarkably compact sequence spanning nucleotides -132 to +21 of Fabpl is sufficient to establish and maintain a distribution of reporter mRNA and protein in villus-associated enterocytes located along the duodenal-to-ileal axis of the gut that resembles the pattern of expression of the endogenous Fabpl gene. L-FABP-132 to +21/hGH+3 is also expressed in surface and pit mucous cells of gastric units and in enterocytes located in the colonic homologs of small intestinal villi, the surface epithelial cuffs. This pattern of transgene expression in the stomach and colon recapitulates that of the intact endogenous donor rat Fabpl but not that of mouse Fabpl, which is silent in these proximal and distal segments of the gastrointestinal tract. Analysis of mice containing L-FABP-4000 to +21/hGH+3, L-FABP-1600 to +21/hGH+3, L-FABP-596 to +21/hGH+3, L-FABP-246 to +21/hGH+3, and L-FABP-186 to +21/hGH+3 indicate that Fabpl's cephalocaudal gradient is influenced by cis-acting suppressors of cecal and colonic expression located between nucleotides -4000 and -1600 and by cis-acting activators of cecal and colonic expression located between nucleotides -597 and -351. L-FABP-132 to +21/hGH+3 is precociously activated in proliferating and nonproliferating epithelial cells located in intestinal crypts. The suppressor(s) of L-FABP accumulation in crypt epithelial cell populations are not represented between nucleotides -4000 and +21, indicating that different cis-acting sequences regulate regional and differentiation-dependent patterns of Fabpl expression.(ABSTRACT TRUNCATED AT 400 WORDS)
尽管哺乳动物肠道上皮的四种主要细胞谱系快速且持续更新,但轴向模式形成仍得以维持。小鼠和大鼠肝脏脂肪酸结合蛋白(L-FABP)基因(Fabpl)是理解决定沿肠道隐窝至绒毛轴以及十二指肠至回肠轴,乃至肝腺泡内依赖分化、细胞谱系特异性和独特区域表达模式机制的绝佳模型。我们利用转基因小鼠来定位大鼠Fabpl中控制这些基因表达模式的顺式作用元件。分析了七个转基因,它们代表从核苷酸+3开始与人生长激素(hGH)基因相连的Fabpl 5'-非转录结构域的连续缺失(L-FABP/hGH+3)。在出生后第8周和第20周结束时,使用免疫细胞化学和RNA杂交分析检查了含有每个L-FABP/hGH+3转基因的几个小鼠谱系。一个跨越Fabpl核苷酸-132至+21的非常紧凑的序列足以在沿肠道十二指肠至回肠轴的绒毛相关肠细胞中建立并维持报告基因mRNA和蛋白质的分布,其类似于内源性Fabpl基因的表达模式。L-FABP-132至+21/hGH+3在胃单位的表面和隐窝黏液细胞以及位于小肠绒毛的结肠同源物即表面上皮袖套中的肠细胞中也有表达。这种转基因在胃和结肠中的表达模式概括了完整内源性供体大鼠Fabpl的表达模式,但并非小鼠Fabpl的表达模式,小鼠Fabpl在胃肠道的这些近端和远端节段中是沉默的。对含有L-FABP-4000至+21/hGH+3、L-FABP-1600至+21/hGH+3、L-FABP-596至+21/hGH+3、L-FABP-246至+21/hGH+3和L-FABP-186至+21/hGH+3的小鼠的分析表明,Fabpl的头尾梯度受位于核苷酸-4000和-1600之间的盲肠和结肠表达的顺式作用抑制因子以及位于核苷酸-597和-351之间的盲肠和结肠表达的顺式作用激活因子的影响。L-FABP-132至+21/hGH+3在位于肠道隐窝的增殖和非增殖上皮细胞中被过早激活。隐窝上皮细胞群体中L-FABP积累的抑制因子在核苷酸-4000和+21之间未体现,这表明不同的顺式作用序列调节Fabpl表达的区域和依赖分化的模式。(摘要截断于400字)
