Khadija Syeda, Veluthakal Rajakrishnan, Sidarala Vaibhav, Kowluru Anjaneyulu
B-4237 Research Service, β-Cell Biochemistry Laboratory, John D. Dingell VA Medical Center, 4646 John R, Detroit, MI, 48201, USA.
Apoptosis. 2014 Dec;19(12):1691-701. doi: 10.1007/s10495-014-1038-4.
Nuclear lamins form the lamina on the interior surface of the nuclear envelope, and regulate nuclear metabolic events, including DNA replication and organization of chromatin. The current study is aimed at understanding the role of executioner caspase 6 on lamin A integrity in islet β-cells under duress of glucotoxic (20 mM glucose; 24 h) and diabetic conditions. Under glucotoxic conditions, glucose-stimulated insulin secretion and metabolic cell viability were significantly attenuated in INS-1 832/13 cells. Further, exposure of normal human islets, rat islets and INS-1 832/13 cells to glucotoxic conditions leads to caspase 6 activation and lamin A degradation, which is also observed in islets from the Zucker diabetic fatty rat, a model for type 2 diabetes (T2D), and in islets from a human donor with T2D. Z-Val-Glu-Ile-Asp-fluoromethylketone, a specific inhibitor of caspase 6, markedly attenuated high glucose-induced caspase 6 activation and lamin A degradation, confirming that caspase 6 mediates lamin A degradation under high glucose exposure conditions. Moreover, Z-Asp-Glu-Val-Asp-fluoromethylketone, a known caspase 3 inhibitor, significantly inhibited high glucose-induced caspase 6 activation and lamin A degradation, suggesting that activation of caspase 3 might be upstream to caspase 6 activation in the islet β-cell under glucotoxic conditions. Lastly, we report expression of ZMPSTE24, a zinc metallopeptidase involved in the processing of prelamin A to mature lamin A, in INS-1 832/13 cells and human islets; was unaffected by high glucose. We conclude that caspases 3 and 6 could contribute to alterations in the integrity of nuclear lamins leading to metabolic dysregulation and failure of the islet β-cell.
核纤层蛋白在核膜内表面形成核纤层,并调节核代谢事件,包括DNA复制和染色质组织。当前的研究旨在了解在糖毒性(20 mM葡萄糖;24小时)和糖尿病条件的胁迫下,凋亡执行蛋白酶6对胰岛β细胞中核纤层蛋白A完整性的作用。在糖毒性条件下,INS-1 832/13细胞中葡萄糖刺激的胰岛素分泌和代谢细胞活力显著减弱。此外,正常人胰岛、大鼠胰岛和INS-1 832/13细胞暴露于糖毒性条件下会导致半胱天冬酶6激活和核纤层蛋白A降解,这在2型糖尿病(T2D)模型 Zucker糖尿病脂肪大鼠的胰岛以及一名T2D人类供体的胰岛中也有观察到。半胱天冬酶6的特异性抑制剂Z-Val-Glu-Ile-Asp-氟甲基酮显著减弱了高糖诱导的半胱天冬酶6激活和核纤层蛋白A降解,证实了半胱天冬酶6在高糖暴露条件下介导核纤层蛋白A降解。此外,已知的半胱天冬酶3抑制剂Z-Asp-Glu-Val-Asp-氟甲基酮显著抑制了高糖诱导的半胱天冬酶6激活和核纤层蛋白A降解,表明在糖毒性条件下,胰岛β细胞中半胱天冬酶3的激活可能在半胱天冬酶6激活的上游。最后,我们报道了参与前核纤层蛋白A加工成成熟核纤层蛋白A的锌金属肽酶ZMPSTE24在INS-1 832/13细胞和人类胰岛中的表达;不受高糖影响。我们得出结论,半胱天冬酶3和6可能导致核纤层蛋白完整性改变,从而导致代谢失调和胰岛β细胞功能衰竭。