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羊膜内注射蛋氨酸锌后鸡肠道锌转运蛋白mRNA表达及小肠功能的变化

Changes in chicken intestinal zinc exporter mRNA expression and small intestinal functionality following intra-amniotic zinc-methionine administration.

作者信息

Tako Elad, Ferket Peter R, Uni Zehava

机构信息

Department of Animal Sciences, The Faculty of Agricultural, Food and Environmental Quality Sciences, The Hebrew University of Jerusalem, P.O. Box 12, Rehovot 76100, Israel.

出版信息

J Nutr Biochem. 2005 Jun;16(6):339-46. doi: 10.1016/j.jnutbio.2005.01.002.

Abstract

A 303-bp cDNA of intestinal zinc exporter (ZnT1) was isolated from chicken jejunum by reverse transcriptase-polymerase chain reaction and sequenced, and showed 42% homology to Homo sapiens and Rattus novergicus intestinal ZnT1 genes. This specific probe was used to examine the effect of zinc-methionine (ZnMet) administration on the mRNA expression of ZnT1 and on small intestinal development and functionality. In this study, ZnMet was injected into the naturally consumed amniotic fluid of 17-day-old chicken embryos. The ZnT1 gene showed an approximately 200% increase in its mRNA levels from 48 h post-ZnMet injection, as compared to the control. An analysis of the gene expression of the brush-border enzymes and transporters showed increased mRNA expression of sucrase isomaltase, leucine-aminopeptidase, sodium-glucose cotransporter and Na+K+ATPase transporter (Na+K+ATPase) from 48 h post-ZnMet injection, in comparison to controls. Significant increases (P<.05) in the biochemical activity of the brush-border enzymes and transporters, and in jejunal villus surface area were detected from day of hatch (96 h post-ZnMet injection) as compared to controls. These results suggest that ZnMet administration into prenatal intestine via injection into the amniotic fluid enhances intestinal development and improves its functionality.

摘要

通过逆转录聚合酶链反应从鸡空肠中分离出肠道锌转运蛋白(ZnT1)的一段303个碱基对的cDNA并进行测序,结果显示其与人类和褐家鼠肠道ZnT1基因有42%的同源性。使用该特异性探针来检测蛋氨酸锌(ZnMet)给药对ZnT1 mRNA表达以及小肠发育和功能的影响。在本研究中,将ZnMet注射到17日龄鸡胚自然摄取的羊水中。与对照组相比,ZnT1基因在注射ZnMet后48小时其mRNA水平增加了约200%。对刷状缘酶和转运蛋白的基因表达分析表明,与对照组相比,注射ZnMet后48小时蔗糖酶异麦芽糖酶、亮氨酸氨肽酶、钠葡萄糖共转运蛋白和Na+K+ATP酶转运蛋白(Na+K+ATPase)的mRNA表达增加。与对照组相比,从孵化日(注射ZnMet后96小时)开始检测到刷状缘酶和转运蛋白的生化活性以及空肠绒毛表面积显著增加(P<0.05)。这些结果表明,通过向羊水中注射将ZnMet给予产前肠道可促进肠道发育并改善其功能。

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