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The technique of simultaneous recording calcium transients and spontaneous transient outward currents in arterial smooth muscle cells

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ã€Authorã€‘ LI Peng-Yun, ZENG Xiao-Rong, LEI Ming, LIU Zhi-Fei, YANG Yan* Institute of Cardiovasology, Luzhou Medical College, Luzhou 646000, China

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ã€Abstractã€‘ Laser scanning confocal microscopy (LSCM) and whole-cell perforated patch-clamp techniques were combined to study simultaneously the changes of intracellular signal molecules and membrane currents. Intracellular calcium transients and spontaneous transient outward currents (STOCs) were recorded simultaneously in freshly isolated mouse cerebral artery smooth muscle cells. The cells loaded with fluo-4/AM were scanned with the confocal line-scan mode. Triggering voltage pulses derived from an EPC-10 patch clamp amplifier triggered the confocal line scan. The results showed that STOCs and intracellular calcium transients could be simultaneously recorded in the same cell. This technique will be useful in studies of diseases caused by impairments of intracellular Ca2+ signaling and related ionic channel activities, or vice versa.æ›´å¤š è¿˜åŽŸ

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ã€Key wordsã€‘ laser scanning confocal microscopyï¼› patch clamp techniqueï¼› spontaneous transient outward currentï¼› Ca2+ transientsï¼›

ã€åŸºé‡‘ã€‘ supported by the National Natural Science Foundation of China(No.30670763);the Scientific Research Fund of Education Department of Sichuan Province,China(No.2006ZD020)

ã€æ–‡çŒ®å‡ºå¤„ã€‘ ç”Ÿç†å¦æŠ¥ ,Acta Physiologica Sinica , ç¼–è¾‘éƒ¨é‚®ç®± ,2010å¹´03æœŸ

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