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Cloning of a pig homologue of the human lactoferrin receptor: Expression and localization during intestinal maturation in piglets

机译:人乳铁蛋白受体的猪同源物的克隆:仔猪肠道成熟过程中的表达和定位

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摘要

The presence of a small intestinal lactoferrin receptor (SI-LfR) has been suggested in the pig, but remains to be identified. LfR has been suggested to play a key role in the internalization of lactoferrin (Lf) and to facilitate absorption of iron bound to Lf. The aim of this study was to identify the pig SI-LfR cDNA, determine its mRNA and protein expression during different stages of intestinal development. The coding region of the pig LfR cDNA was cloned by PCR using conserved sequences among species. LfR mRNA expression and protein abundance were measured in proximal small intestine from piglets at 1 week (pre-weaning), 3 weeks (weaning) and 6 months (post-weaning) of age by quantitative (real-time) RT-PCR (Q-PCR) and Western blot, respectively. Intestinal brush border membrane vesicles (BBMV) were also isolated to examine LfR abundance on the apical membrane. We determined the pig SI-LfR open reading frame (ORF) consists of 972 bp, resulting in a protein with a molecular mass ~135 kD and ~35 kD under non-reducing and reducing conditions, respectively. Using Q-PCR, we determined LfR expression significantly increased with age in the duodenum and reciprocally decreased in the jejunum. Intestinal LfR protein expression was maintained at all timepoints in the jejunum; however, in the duodenum LfR abundance reached maximum levels at 6 months. In BBMV fractions, LfR abundance significantly increased with age. Taken together our findings demonstrate the presence of a human SI-LfR homologue in pig, with mRNA and protein expression concomitantly regulated in the duodenum and inversely regulated in the jejunum. These findings suggest a mechanism by which pig Lf can be internalized in the intestine.
机译:有人建议在猪中存在小肠乳铁蛋白受体(SI-LfR),但仍有待确定。已经建议LfR在乳铁蛋白(Lf)的内在化中起关键作用,并促进与Lf结合的铁的吸收。这项研究的目的是鉴定猪SI-LfR cDNA,确定其在肠道发育不同阶段的mRNA和蛋白表达。利用物种间的保守序列,通过PCR克隆了猪LfR cDNA的编码区。通过定量(实时)RT-PCR(断奶),在1周龄(断奶前),3周龄(断奶)和6个月龄(断奶后)的仔猪近端小肠中测量LfR mRNA表达和蛋白丰度。 -PCR)和蛋白质印迹。还分离了肠刷状缘膜囊泡(BBMV)以检查LfR在顶膜上的丰度。我们确定了猪SI-LfR开放阅读框(ORF)由972 bp组成,分别在非还原和还原条件下产生的蛋白质的分子量分别约为135 kD和〜35 kD。使用Q-PCR,我们确定LfR表达在十二指肠中随着年龄的增长而显着增加,而在空肠中则相反。空肠在所有时间点均保持肠道LfR蛋白表达。然而,十二指肠中LfR的丰度在6个月时达到最高水平。在BBMV分数中,LfR丰度随着年龄的增长而显着增加。综上所述,我们的发现表明猪中存在人SI-LfR同源物,mRNA和蛋白表达在十二指肠中同时受到调节,而在空肠中则受到相反的调节。这些发现提示了猪Lf可以在肠道内被内化的机制。

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