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首页 > 过刊浏览>2017年第27卷第7期 >17-23. DOI:10.3969.j.issn.1671-7856.2017.07.004
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改良的两步复合酶消化法制备大鼠胸主动脉血管平滑肌细胞
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国家自然科学基金(编号:81371675,81330031)。


Preparation of rat thoracic aortic vascular smooth muscle cells by modified enzyme double digestion
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    摘要:

    目的 本文报道一种基于复合酶消化法进行改良的大鼠胸主动脉血管平滑肌细胞的分离方法。方法 采用胶原酶、胰肽酶复合酶对胸主动脉进行初步消化去除内外膜、再对中膜进行二次消化释放血管平滑肌细胞。结果 细胞分离后贴壁生长,多具梭形形态,呈现典型的“峰-谷”生长状态,1周可进行传代;多种收缩型血管平滑肌细胞的分子标记基因均在所分离培养的细胞中高表达;超过95%的细胞为alpha smooth muscle actin(α-SMA)和myosin-Ⅱ显著阳性。结论 本分离方法简捷易行、重复性好,所得细胞活性佳、纯度高,可确保短时间内获得大量收缩型血管平滑肌细胞。

    Abstract:

    Objective This paper reports a modified method for the isolation of rat thoracic aortic vascular smooth muscle cells based on combined enzyme double digestion. Methods An enzyme mixture containing collagenase Ⅱ, soybean trypsin inhibitor and elastase was prepared and used to remove the aortic tunica intima and tunica adventitia, and then the tunica media was subjected to second digestion using the same enzyme mixture and to isolate vascular smooth muscle cells. Results The isolated VSMCs were cultured in vitro and the growing cells had an elongated spindle-shape, reached confluence within a week, and displaying a typical "hill-and-valley" pattern. After 1 week, the cells were passaged. Contractile smooth muscle markers(α-SMA, myosin-Ⅱ and β-tubulin) were highly expressed in the isolated cells. More than 90% of the cells significantly expressed alpha smooth muscle actin and myosin-Ⅱ. Conclusions Themethod established in this study has advantages of simple and easy to operate, and good reproducibility, with a high activity and purity of the separated cells. It can ensure to obtain a large amount of contraction-type vascular smooth muscle cells within a short time.

    参考文献
    [1] 王生兰,刘辉琦,王丽华,等.酶消化法分离培养家兔血管平滑肌细胞[J]. 青海医学院学报, 2008, 29(4):249-252.
    [2] 刘红梅,黄体钢.血管平滑肌细胞的培养及其在心血管疾病研究中的应用[J]. 实用心脑肺血管病杂志, 2005, 13(6):364-68.
    [3] Owens GK.Molecular regulation of vascular smooth muscle cell differentiation in development and disease[J].Physiol Rev, 2004,84(3):767-801.
    [4] 丁洪飞,黄胜超,李建文,等.改良大鼠血管平滑肌细胞的原代培养[J].医学研究杂志, 2011, 40(1):71-73.
    [5] Freed D.Induction of protein synthesis in cardiac fibroblasts by cardiotrophin-1:integration of multiple signaling pathways[J].Cardiovasc Res,2003,60(2):365-75.
    [6] Tsuruda T.Cardiotrophin-1 stimulation of cardiac fibroblast growth:roles for glycoprotein 130/leukemia inhibitory factor receptor and the endothelin type A receptor[J].CIRC RES,2002,90(2):128-134.
    [7] 卓致远,黄茂,崔学范,等.组织贴块法培养小鼠气道平滑肌细胞[J].中国组织化学与细胞化学杂志, 2007, 16(2):247-50.
    [8] 吴海亚,戴元荣,尹娟. 改良组织贴块法培养大鼠气道平滑肌细胞[J]. 温州医学院学报, 2010, 40(6):571-73.
    [9] 叶致豪,许文豪,刘庆华,等. 小鼠气管平滑肌原代细胞的分离、培养与鉴定[J].中国实验动物学报, 2016, 24(4):364-368.
    [10] 张正杨,王含彦,易芳,等.小鼠原代血管平滑肌细胞改良分离方法的建立.海南医学院学报[J]. 2014, 20(3):302-312.
    [11] Asrih M,Mach F,Quercioli A,et al.Update on the pathophysiological activities of the cardiac molecule cardiotrophin-1 in obesity[J].Mediat Inflamm,2013, 2013:Article ID 370715.
    [12] 周晓莉,雷寒,柳青.血管平滑肌细胞的培养及鉴定[J].重庆医学, 2005, 34(6):877-878.
    [13] Siow RC, Pearson JD. Vascular smooth muscle cells:isolation, culture, and characterization[J]. Methods MolMed, 2001, 46:237-245.
    [14] Parmacek MS. Myocardin:Dominant driver of the smooth muscle cell contractile phenotype[J]. Arterioscler Thromb Vasc Biol,2008,28(8):1416-1417.
    [15] Ives HE, Schultz GS, Galardy RE, et al. Preparation of functional smooth muscle cells from the rabbit aorta[J]. J ExpMed, 1978, 148(5):1400-1413.
    [16] 辛毅,张耀中,林筝,等.小鼠主动脉血管平滑肌细胞分离培养及鉴定[J]. 新乡医学院学报, 2012, 29(1):5-10.
    [17] Kim KG, Sung EG, Kim JY. An effective isolation of the vascular endothelial and smooth muscle cells from the mouse aorta[J]. Korean J Anat, 2009, 42(2):93-104.
    [18] 王志勇,邹祖玉,刘维新.血管平滑肌细胞的表型标志α-SM-actin的表达与调控的研究进展[J]. 数理医药学杂志, 2001, 14(05):443-445.
    [19] 涂永生,黄红林,朱炳阳,等.Ⅱ型胶原酶/弹性蛋白酶消化法培养大鼠血管平滑肌细胞[J]. 中国动脉硬化杂志, 2001, 9(5):438-440.
    [20] Shunsuke M,Wataru N, Mako N,et al.Role of Bagpipe, a member of NK homeobox genes,in regulating smooth muscle-specific expression of SM22α[C].Third Congress of the Asian-Pacific Organization for Cell Biology, 日本大阪,1998:1.
    [21] 李宪伟,姜维良.酶消化法分离培养大鼠血管平滑肌细胞方法的改良[J].哈尔滨医科大学学报, 2011, 45(1):58-60, 63.
    [22] Geisterfer AA, Peach MJ, Owens GK. et al. Angiotensin Ⅱ induces hypertrophy,not hyperplasia,of cultured rat aortic smooth muscle cells[J].Circ Res,1988,62:749-756.
    [23] Gunther S, Alexander RW, Atkinson WJ, et al.Functional angiotensin Ⅱ receptors in cultured vascular smooth muscle cells[J].J Cell Biol,1982,92(2):289-298.
    [24] Owens GK, Loeb A, Gordon D, et al.Expression of smooth muscle-specific alpha-isoactin in cultured vascular smooth muscle cells:relationship between growth and cytodifferentiation[J].J Cell Biol, 1986,102(2):343-352.
    [25] Ray JL,Leach R,Herbert JM,et al.Isolation of vascular smooth muscle cells from a single murine aorta[J]. Methods Cell Sci,2001,23(4):185-188.
    [26] Kobayashi M,Inoue K,Warabi E,et al.A simple method of isolating mouse aortic endothelial cells[J].J Atheroscler Thromb,2005, 12(3):138-142.
    [27] Gomez D,Owens GK.Smooth muscle cell phenotypic switching in atherosclerosis[J]. Cardiovasc Res,2012,95(2):1561-1564.
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周玥华,刘星,张艳军,汪辛,陈渝萍.改良的两步复合酶消化法制备大鼠胸主动脉血管平滑肌细胞[J].中国比较医学杂志,2017,27(7):17~23.

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  • 最后修改日期:2016-12-05
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