Krüger Martina, Sachse Christine, Zimmermann Wolfram H, Eschenhagen Thomas, Klede Stefanie, Linke Wolfgang A
Physiology and Biophysics Unit, University of Muenster, Schlossplatz 5, D-48149 Muenster, Germany.
Circ Res. 2008 Feb 29;102(4):439-47. doi: 10.1161/CIRCRESAHA.107.162719. Epub 2007 Dec 20.
Titins, giant sarcomere proteins with major mechanical/signaling functions, are expressed in 2 main isoform classes in the mammalian heart: N2B (3000 kDa) and N2BA (>3200 kDa). A dramatic isoform switch occurs during cardiac development, from fetal N2BA titin (3700 kDa) expressed before birth to a mix of smaller N2BA/N2B isoforms found postnatally; adult rat hearts almost exclusively have N2B titin. The isoform switch, which can be reversed in chronic human heart failure, alters myocardial distensibility and mechanosignaling. Here we determined factors regulating this switch using, as a model system, primary cardiomyocyte cultures prepared from embryonic rats. In standard culture, the mean N2B percentage initially was 14% and increased by approximately 60% within 1 week, resembling the in vivo switching. The titin isoform transition was independent of endothelin-1-induced myocyte hypertrophy and was not altered by pacing, contractile arrest, or cell stretch; however, it was modestly impaired by decreasing substrate rigidity and strongly dependent on serum components. Angiotensin II significantly promoted the transition. The mean N2B proportion in 1-week-old cultures dropped 20% to 25% in hormone-reduced medium, but addition of 3,5,3'-triiodo-l-thyronine (T3) nearly restored the proportion to that found in standard culture. This T3 effect was not prevented by bisphenol A, a specific inhibitor of the classic genomic pathway of T3 action. In contrast, the titin switch could be stalled by the phosphatidylinositol 3-kinase inhibitor LY294002, which decreased the proportion of N2B mRNA transcripts within hours and suppressed a rapid T3-induced increase in Akt phosphorylation. Also, angiotensin II, but not endothelin-1 or cell stretch, enhanced Akt phosphorylation. Thus, although matrix stiffness modulates developmental titin isoform transitions, these transitions are mainly regulated through phosphatidylinositol 3-kinase/Akt-dependent signaling triggered particularly by T3 via a rapid action pathway.
肌联蛋白是具有主要机械/信号功能的巨大肌节蛋白,在哺乳动物心脏中以两种主要的异构体形式表达:N2B(3000 kDa)和N2BA(>3200 kDa)。在心脏发育过程中会发生显著的异构体转换,从出生前表达的胎儿N2BA肌联蛋白(3700 kDa)转换为出生后发现的较小的N2BA/N2B异构体混合物;成年大鼠心脏几乎只含有N2B肌联蛋白。这种异构体转换在慢性人类心力衰竭中可以逆转,它会改变心肌的伸展性和机械信号传导。在这里,我们以从胚胎大鼠制备的原代心肌细胞培养物为模型系统,确定了调节这种转换的因素。在标准培养中,N2B的平均百分比最初为14%,并在1周内增加了约60%,类似于体内的转换。肌联蛋白异构体的转变与内皮素-1诱导的心肌细胞肥大无关,并且不受起搏、收缩停止或细胞拉伸的影响;然而,通过降低底物硬度会适度损害这种转变,并且它强烈依赖于血清成分。血管紧张素II显著促进了这种转变。在激素减少的培养基中,1周龄培养物中N2B的平均比例下降了20%至25%,但添加3,5,3'-三碘-L-甲状腺原氨酸(T3)几乎将该比例恢复到标准培养中的水平。双酚A是T3作用经典基因组途径的特异性抑制剂,它并不能阻止这种T3效应。相反,磷脂酰肌醇3-激酶抑制剂LY294002可以使肌联蛋白转换停滞,该抑制剂在数小时内降低了N2B mRNA转录本的比例,并抑制了T3诱导的Akt磷酸化的快速增加。此外,血管紧张素II增强了Akt磷酸化,而内皮素-1或细胞拉伸则没有。因此,尽管基质硬度调节发育过程中的肌联蛋白异构体转换,但这些转换主要通过磷脂酰肌醇3-激酶/Akt依赖性信号传导来调节,特别是由T3通过快速作用途径触发。
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