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作 者:顾霞[1] 吴健[1] 谭妙欣[1] 李振超[1] 韩娜[1] 曹瑞[1] 孙勇[1]
机构地区:[1]哈尔滨医科大学附属第二医院心内科,心肌缺血省部共建教育部重点实验室,黑龙江哈尔滨150081
出 处:《中国心脏起搏与心电生理杂志》2014年第4期345-348,共4页Chinese Journal of Cardiac Pacing and Electrophysiology
基 金:国家自然科学基金青年基金(编号:81200240);黑龙江省青年基金(编号:QC2010048);中国博士后特别资助(编号:2013T60391)
摘 要:目的研究不同人来源的人左心耳组织培养的c-kit+(CD117)心脏干细胞(c-kit+CSCs)的离子通道的表达情况,进一步了解心脏干细胞的电生理特性,为临床干细胞移植的安全性提供参考。方法通过分离筛选培养人c-kit+CSCs,运用全细胞膜片钳和定量反转录聚合酶连锁反应(qRT-PCR)技术,检测人c-kit+CSCs的通道电流和MaxiK基因、HNE-Na基因、CACNA1G基因、Kv4.2基因、CACNA1C基因的表达情况。结果在人c-kit+CSCs上,记录到了人电压依赖性Ca2+激活K+电流,检测到MaxiK基因表达相对较高,HNE-Na基因、CACNA1G基因表达尚可,Kv4.2基因通道的表达相对较低,未见CACNA1C基因的表达。结论人c-kit+CSCs表达多种离子通道的相关基因,能记录到人电压依赖性Ca2+激活K+电流,这与其基因的高表达是相一致的。Objective To investigate functional ion channels in undifferentiated human c-kit (CDl17) cardiac stem cells (c-kit+ CSCs), learn more about cardiac stem cell electrophysiological characteristics for the purpose of clinical stem cell transplantation security. Methods Isolation of cultured human c-kit+ CSCs, using whole-cell patch clamp and quan- titative reverse transcription polymerase chain reaction (qRT-PCR) technology to detect human c-kit+ CSCs channel cur- rents and the expression of MaxiK gene, HNE-Na gene, CACNA1G gene, hKv4.2 gene, CACNA1C gene. Results In the human c-kit+ CSCs, the whole-cell patch clamp technique to human voltage-dependent Ca activated K+ current, qRT- PCR gene expression detected MaxiK relatively high, HNE-Na gene, CACNA1G gene expression is acceptable, hKv4. 2 gene expression in the channel is relatively low, no CACNA1C gene expression. Conclusion C-kit+ CSCs express variety of ion channel genes, it can be recorded through the human voltage-dependent Ca2+ activated K+ current, which is consistent with gene's high expression.
分 类 号:R331.38[医药卫生—人体生理学]
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