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内皮细胞特异性 Hrh2 敲除小鼠的建立与鉴定。

Generation and identification of endothelial-specific Hrh2 knockout mice.

机构信息

Department of Clinical Pharmacy, 920th Hospital of Joint Logistics Support Force, 212 Daguan Rd, Kunming, 650032, China.

Kunming Medical University, Kunming, 650500, China.

出版信息

Transgenic Res. 2021 Jun;30(3):251-261. doi: 10.1007/s11248-021-00244-z. Epub 2021 Mar 30.

DOI:10.1007/s11248-021-00244-z
PMID:33786748
Abstract

Histamine H receptor (HRH2) is closely associated with the development of cardiovascular and cerebrovascular diseases. However, systematic Hrh2 knockout mice did not exactly reflect the HRH2 function in specific cell or tissue types. To better understand the physiological and pathophysiological functions of endothelial HRH2, this study constructed a targeting vector that contained loxp sites flanking the ATG start codon located in Hrh2 exon 2 upstream and a neomycin (Neo) resistance gene flanked by self-deletion anchor sites within the mouse Hrh2 allele. The targeting vector was then electroporated into C57BL/6J embryonic stem (ES) cells, and positively targeted ES cell clones were micoinjected into C57BL/6J blastocysts, which were implanted into pseudopregnant females to obtain chimeric mice. The F1 generation of Hrh2 mice was generated via crossing chimeric mice with wild-type mice to excise Neo. We also successfully generated endothelial cell-specific knockout (ECKO) mice by crossing Hrh2 mice with Cdh5-Cre mice that specifically express Cre in endothelial cells and identified that Hrh2 deletion was only observed in endothelial cells. Hrh2 and Hrh2 mice were normal, healthy and fertile and did not display any obvious abnormalities. These novel animal models will create new prospects for exploring roles of HRH2 during the development and treatment of related diseases.

摘要

组胺 H 受体(HRH2)与心血管和脑血管疾病的发展密切相关。然而,系统敲除 Hrh2 的小鼠并不能完全反映特定细胞或组织类型中 HRH2 的功能。为了更好地理解内皮细胞 HRH2 的生理和病理生理功能,本研究构建了一个靶向载体,该载体包含侧翼位于 Hrh2 外显子 2 的 ATG 起始密码子的 loxp 位点和在小鼠 Hrh2 等位基因内的自我缺失锚定位点侧翼的新霉素(Neo)抗性基因。然后将靶向载体电穿孔到 C57BL/6J 胚胎干细胞(ES 细胞)中,并将阳性靶向 ES 细胞克隆微注射到 C57BL/6J 囊胚中,将囊胚植入假孕雌性中以获得嵌合小鼠。通过将嵌合小鼠与野生型小鼠杂交来产生 Hrh2 小鼠的 F1 代以切除 Neo。我们还通过将 Hrh2 小鼠与 Cdh5-Cre 小鼠杂交成功地产生了内皮细胞特异性敲除(ECKO)小鼠,该小鼠在内皮细胞中特异性表达 Cre,并且鉴定出 Hrh2 缺失仅发生在内皮细胞中。Hrh2 和 Hrh2 小鼠正常、健康且有生育能力,没有表现出任何明显的异常。这些新型动物模型将为探索 HRH2 在相关疾病的发展和治疗中的作用开辟新的前景。

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