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¡¶ÐÄÔàÔÓÖ¾¡·[ISSN:1009-7236/CN:61-1268/R]

ÆÚÊý:

2006ÄêµÚ3ÆÚ

Ò³Âë:

258-261

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2006-06-25

ÎÄÕÂÐÅÏ¢/Info

Title:

Angiotensin¢ò induces cardiomyocytes from human bone marrow-derived mesenchymal stem cells

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µÚËľüÒ½´óѧÎ÷¾©Ò½ÔºÐÄѪ¹ÜÄÚ¿Æ£¬ ÉÂÎ÷ Î÷°² 710032

Author(s):

YUAN Yuan;  Lv An-lin;  CHEN Dan;  DIAO Fan-rong;  LI Jun-jie;  HU Xiao-jing;  YI Fu

Department of Cardiology, Xijing Hospital, Fourth Military Medical University, Xi¡äan,Shaanxi 710032, China

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¹ÇËè¼ä³äÖʸÉϸ°û; Ðļ¡Ñùϸ°û; Ñª¹Ü½ôÕÅËØ¢ò

Keywords:

bone marrow-derived mesenchymal stem cells; cardiomyocyte; angiotensin¢ò

·ÖÀàºÅ:

R331.31

DOI:

-

ÎÄÏ×±êʶÂë:

A

ÕªÒª:

Ä¿µÄ Ñо¿Ñª¹Ü½ôÕÅËØ¢ò(Ang¢ò)×÷ÓÃÓÚÈ˹ÇËè¼ä³äÖʸÉϸ°û(hMSCs)ºó£¬Ðļ¡ÌØÒìµ°°×¼°Ï¸°ûÍâÐźŵ÷½Ú¼¤Ã¸£¨ERK 1£¯2£©µÄ±í´ï±ä»¯¡£·½·¨ µÚ8´úhMSCsÓÃ0.1 ¦Ìmol/L Ang¢ò·õÓý24 h¡£µ¹ÖÃÏÔ΢¾µÏ¹۲ìϸ°ûÐÎ̬±ä»¯,ÃâÒßϸ°û»¯Ñ§·¨±ê²âÐļ¡¼¡¸Æµ°°×I(cTnI)¡¢¼ä϶Á¬½Óµ°°×43£¨connexin 43£©¼°¦Á¼¡¶¯µ°°×(¦Áª²actin)±í´ïÇé¿ö,·´×ªÂ¼PCR·¨¼ì²âϸ°ûcTnI±í´ï£¬Í¸Éäµç¾µ¹Û²ì·Ö»¯µÄÐļ¡Ñùϸ°ûÄÚÊÇ·ñÓм¡Ë¿´æÔÚ£¬Western blot·¨¼ì²âϸ°ûERK 1£¯2×ܵ°°×±í´ï,Á÷ʽϸ°ûÒDzⶨÐļ¡Ñùϸ°û·Ö»¯ÂÊ¡£½á¹û Óë¶ÔÕÕ×é±È½Ï£¬Ang¢ò×éhMSCsÓÕµ¼ºóϸ°ûÐÎ̬¸Ä±ä£¬µÚ2ÖÜ¿ªÊ¼±í´ï¦Áª²actin¼°connexin 43£¬µÚ3ÖÜ¿ªÊ¼±í´ïcTnI£¬Ang¢ò×éϸ°ûERK 1£¯2µÄµ°°×±í´ïˮƽÖð½¥Ôö¼Ó£¬Á÷ʽϸ°ûÒDzâµÃÐļ¡Ñùϸ°û·Ö»¯ÂÊΪ(23¡À3)£¥¡£½áÂÛ Ang¢òÔÚÌåÍâ¿ÉÄܾ­ERKͨ·ÓÕµ¼hMSCÏòÐļ¡Ñùϸ°û·Ö»¯¡£

Abstract:

AIM To investigate the changes of specific protein of myocardium and extracellular signal regulated kinase 1£¯2(ERK1£¯2) of human bone marrowª²derived mesenchymal stem cells (hMSCs) induced to cardiomyocytes in vitro with the treatment of angiotensin¢ò (Ang¢ò). METHODS 4 ml of bone marrow was obtained from normal adults and hMSCs were isolated by proportion 1.077 Ficoll and were cultured in LGª²DMEM for more than 8 passage. hMSCs were treated with 0.1 ¦Ìmol/L Ang¢ò for 24 hours. The differentiation of MSCs was observed with a phaseª²contrast mictmcope. The induced cells were evaluated by immunocytochemistry staining and RTª²PCR analysis, and the myofilament structure was observed by electron microscopy observed. The ERKI£¯2 at different time points was measured by Western blot and cardiomyocytes differentiation was examined by flow cytometer. RESULTS After the induction by Ang¢ò, some hMSCs became bigger and longer. The cells were arrayed in a similar direction. The cells induced by Ang¢ò were stained positively for aª²actin, connexin 43 and cTnI. RTª²PCR showed that these cells expressed Cardiac Troponin I. The expression of ERK1£¯2 increased in Ang¢ò group. CONCLUSION Ang¢ò induces human bone marrowª²derived mesenchymal stem cells into cardiomyocytes and ERK1£¯2 MAPK pathway may be involved in cardiomyocytes differentiation of hMSCs cultures.

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