首页> 美国卫生研究院文献>Proceedings of the National Academy of Sciences of the United States of America >Use of transgenic mice to infer the biological properties of small intestinal stem cells and to examine the lineage relationships of their descendants.
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Use of transgenic mice to infer the biological properties of small intestinal stem cells and to examine the lineage relationships of their descendants.

机译:使用转基因小鼠推断小肠干细胞的生物学特性并检查其后代的谱系关系。

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摘要

Transgenes, composed of elements of the 5' nontranscribed region of the liver fatty acid-binding protein (L-FABP) gene linked to various reporters, have previously been used to explore the cellular, regional, and temporal differentiation of the mouse intestinal epithelium. In this report, we have analyzed a pedigree of L-FABP/human growth hormone (hGH) transgenic mice that display a stable, heritable, mosaic pattern of reporter expression: wholly hGH-positive or hGH-negative populations of differentiating enterocytes arise from hGH-positive or hGH-negative crypts, respectively, and migrate as vertical coherent bands up the villus producing striped (polyclonal) villi. The ability of enteroendocrine cells within a given villus stripe to support hGH expression coincides with the enterocytic reporter phenotype, suggesting that these two terminally differentiated cells arise from a common multipotent stem cell. hGH-negative crypts are nonrandomly distributed around each villus and their frequency increases along the duodenal-to-ileal axis. Statistical analysis of the observed villus striping pattern suggests that transgene expression is not independently determined in individual crypts but rather in multicrypt "patches." The intact endogenous mouse L-FABP gene (Fabpl) exhibits a similar striped villus pattern of expression in a portion of the distal small intestine. These studies indicate that Fabpl and L-FABP/hGH transgenes represent sensitive markers for exploring the biological properties of gut stem cells and how positional information is encoded in this rapidly and continuously renewing epithelium.
机译:转基因由与各种报道分子相连的肝脏脂肪酸结合蛋白(L-FABP)基因5'非转录区的元件组成,以前已用于研究小鼠肠上皮的细胞,区域和时间分化。在本报告中,我们分析了谱系稳定的,可遗传的,报道基因表达模式的L-FABP /人类生长激素(hGH)转基因小鼠:分化为完整hGH阳性或hGH阴性的肠细胞群来自hGH -隐窝或hGH阴性隐窝,并以垂直连贯带向绒毛产生条带化(多克隆)绒毛上迁移。给定绒毛区域内肠内分泌细胞支持hGH表达的能力与肠上皮报告基因表型相吻合,表明这两个终末分化的细胞来自共同的多能干细胞。 hGH阴性隐窝在每个绒毛周围非随机分布,其频率沿十二指肠至回肠轴增加。对观察到的绒毛剥离模式的统计分析表明,转基因表达不是在单个隐窝中独立确定的,而是在多重隐窝“补丁”中独立确定的。完整的内源小鼠L-FABP基因(Fabp1)在远端小肠的一部分中表现出相似的条纹绒毛表达模式。这些研究表明,Fabp1和L-FABP / hGH转基因代表了敏感标记,可用于探索肠道干细胞的生物学特性以及在这种快速且持续更新的上皮细胞中如何编码位置信息。

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