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成年动物中的 Ilk 条件性缺失会增加环鸟苷酸依赖性血管舒张。

Ilk conditional deletion in adult animals increases cyclic GMP-dependent vasorelaxation.

机构信息

Faculty of Medicine, Department of Physiology, University of Alcala, Alcalá de Henares, Madrid, Spain.

出版信息

Cardiovasc Res. 2013 Aug 1;99(3):535-44. doi: 10.1093/cvr/cvt131. Epub 2013 May 27.

DOI:10.1093/cvr/cvt131
PMID:23715557
Abstract

AIMS

Integrin-linked kinase (ILK) regulates proliferation, differentiation, cell adhesion, and motility in many cell types and has been related to cancer progression, fibrosis, and vascular diseases. We designed the present study to directly explore the effect of ILK deletion on the regulation of vascular tone through the soluble guanylate cyclase (sGC) /protein kinase G (PKG) pathway in healthy adult mice.

METHODS AND RESULTS

Experiments were carried out using a tamoxifen-inducible CRE-LOX system to conditionally delete the ILK gene in adult mice. Mice lacking ILK expression (cKO) presented increased vascular content and increased activity of sGC and PKG, resulting in a more intense vasodilatory response to a single dose of a nitric oxide (NO) donor [sodium nitroprusside (SNP)] or PKG agonist [8-bromoguanosine 3',5'-cyclic monophosphate sodium salt (8-Br)]. Five minutes after SNP or 8-Br administration the reduction in the systolic arterial pressure was enhanced in cKO mice (SNP WT: -7.4 ± 1.2 mmHG; SNP cKO: -14.0 ± 2.5; 8-Br WT: -2.9 ± 1.5 mmHG; 8-Br cKO: -10.0 ± 3.4 mmHG). ILK deletion restored the vascular response to SNP after chronic oral nitrite administration. In addition, ILK deletion also increased hypotensive SNP effect in angiotensin II-treated animals, suggesting a role for ILK in basal and pathological states.

CONCLUSION

Deletion of ILK in adult animals increased the vascular response to NO. These findings show, for the first time, a requirement for ILK in regulating sGC-PKG expression in vivo.

摘要

目的

整合素连接激酶(ILK)调节许多细胞类型的增殖、分化、细胞黏附和迁移,并且与癌症进展、纤维化和血管疾病有关。我们设计了本研究,旨在通过在健康成年小鼠中使用可诱导的 tamoxifen 型 CRE-LOX 系统直接探索 ILK 缺失对可溶性鸟苷酸环化酶(sGC)/蛋白激酶 G(PKG)通路调节血管张力的影响。

方法和结果

实验使用 tamoxifen 诱导型 CRE-LOX 系统在成年小鼠中条件性删除 ILK 基因。缺乏 ILK 表达的小鼠(cKO)表现出血管含量增加和 sGC 和 PKG 活性增加,导致对一氧化氮(NO)供体[硝普钠(SNP)]或 PKG 激动剂[8-溴鸟苷 3',5'-环单磷酸钠盐(8-Br)]的单次剂量产生更强的血管舒张反应。给予 SNP 或 8-Br 后 5 分钟,cKO 小鼠的收缩压降低更为明显(SNP WT:-7.4±1.2mmHg;SNP cKO:-14.0±2.5mmHg;8-Br WT:-2.9±1.5mmHg;8-Br cKO:-10.0±3.4mmHg)。慢性口服亚硝酸盐给药后,ILK 缺失恢复了 SNP 的血管反应。此外,ILK 缺失还增加了血管紧张素 II 处理动物中 SNP 的降压作用,表明 ILK 在基础和病理状态下发挥作用。

结论

成年动物中 ILK 的缺失增加了对 NO 的血管反应。这些发现首次表明,ILK 在体内调节 sGC-PKG 表达中是必需的。

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