Cardiovascular Division, King's College London, The Rayne Institute, St Thomas' Hospital, London SE1 7EH, UK.
Exp Physiol. 2010 Apr;95(4):518-27. doi: 10.1113/expphysiol.2009.052126. Epub 2010 Jan 8.
In this study, we compared the rate of detubulation of adult mouse and rat ventricular myocytes over a 72 h culture period. The T-tubule density was measured in the following two ways: (i) as whole-cell capacitance in voltage-clamped myocytes relative to cell area; and (ii) using di-8-ANEPPS staining and confocal microscopy. In adult rat ventricular myocytes, whole-cell capacitance/area was significantly reduced from 47 +/- 3 fF microm(2) (mean +/- s.e.m.; n = 16) in freshly isolated (control) cells to 36 +/- 2 fF microm(2) (n = 20) after 72 h in culture. The T-tubular density, as assessed optically using di-8-ANEPPS staining, at 48 h was significantly reduced to 70 +/- 7% (n = 14) compared with control cells. The T-tubular density was further reduced after 72 h in culture to 43 +/- 7% (n = 10) compared with control cells. In contrast, in mouse myocytes neither whole-cell capacitance relative to cell area nor optical assessment of T-tubules showed any significant reduction in capacitance/cell area or T-tubule density after 72 h of culture. Expression of caveolin-3 (CAV-3) (a marker of T-tubule development) was also measured, and a significant reduction was observed in CAV-3 expression in rat myocytes at 48 (80 +/- 5.5%; n = 6) and 72 h (66 +/- 9.5%; n = 6) compared with control cells. The expression of CAV-3 in mouse myocytes was not significantly reduced even at 72 h. When rat ventricular myocytes were paced in culture for 72 h they exhibited no significant improvement in T-tubule density or CAV-3 expression compared with non-paced cultured cells. In rat myocytes, sarcomere length shortening was significantly reduced in myocytes cultured for 48 (4.96 +/- 0.72%; n = 26) and 72 h (4.32 +/- 0.80%; n = 26) compared with freshly isolated cells (7.12 +/- 0.56%; n = 18). Mouse myocytes, after 24 h in culture, were unable to follow external pacing. These results suggest that detubulation in quiescent culture is slower in the mouse than the rat and that this loss of T-tubules profoundly affects excitation-contraction coupling in rat myocytes.
在这项研究中,我们比较了成年小鼠和大鼠心室肌细胞在 72 小时培养过程中的去管化率。通过以下两种方法测量 T 管密度:(i)电压钳制的心肌细胞的全细胞电容相对于细胞面积;和(ii)使用 di-8-ANEPPS 染色和共聚焦显微镜。在成年大鼠心室肌细胞中,全细胞电容/面积从新鲜分离(对照)细胞的 47 +/- 3 fF microm(2)(n = 16)显著降低至 72 h 培养后的 36 +/- 2 fF microm(2)(n = 20)。使用 di-8-ANEPPS 染色光学评估的 T 管密度在 48 h 时显著降低至 70 +/- 7%(n = 14)与对照细胞相比。在培养 72 小时后,T 管密度进一步降低至 43 +/- 7%(n = 10)与对照细胞相比。相比之下,在小鼠心肌细胞中,无论全细胞电容相对于细胞面积还是 T 管的光学评估,在培养 72 小时后,电容/细胞面积或 T 管密度均无明显降低。还测量了 caveolin-3 (CAV-3)(T 管发育的标志物)的表达,与对照细胞相比,在 48 小时(80 +/- 5.5%;n = 6)和 72 小时(66 +/- 9.5%;n = 6)时,大鼠心肌细胞中的 CAV-3 表达显著降低。即使在 72 小时,小鼠心肌细胞中的 CAV-3 表达也没有明显降低。当在培养中起搏大鼠心室肌细胞 72 小时时,与未起搏培养的细胞相比,T 管密度或 CAV-3 表达没有明显改善。在大鼠心肌细胞中,培养 48 小时(4.96 +/- 0.72%;n = 26)和 72 小时(4.32 +/- 0.80%;n = 26)的肌节长度缩短与新鲜分离的细胞(7.12 +/- 0.56%;n = 18)相比显著降低。培养 24 小时后的小鼠心肌细胞无法跟随外部起搏。这些结果表明,在静息培养中,小鼠的去管化速度比大鼠慢,并且这种 T 管的丧失严重影响大鼠心肌细胞的兴奋-收缩偶联。
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