蛋白酶激活受体2(PAR2)在平滑肌中独特的G蛋白依赖性信号传导:非cAMP依赖性蛋白激酶A对RhoA的反馈抑制
Distinctive G Protein-Dependent Signaling by Protease-Activated Receptor 2 (PAR2) in Smooth Muscle: Feedback Inhibition of RhoA by cAMP-Independent PKA.
作者信息
Sriwai Wimolpak, Mahavadi Sunila, Al-Shboul Othman, Grider John R, Murthy Karnam S
机构信息
Department of Physiology, VCU Program in Enteric Neuromuscular Sciences, Virginia Commonwealth University, Richmond, Virginia, United States of America.
出版信息
PLoS One. 2013 Jun 18;8(6):e66743. doi: 10.1371/journal.pone.0066743. Print 2013.
We examined expression of protease-activated receptors 2 (PAR2) and characterized their signaling pathways in rabbit gastric muscle cells. The PAR2 activating peptide SLIGRL (PAR2-AP) stimulated Gq, G13, Gi1, PI hydrolysis, and Rho kinase activity, and inhibited cAMP formation. Stimulation of PI hydrolysis was partly inhibited in cells expressing PAR2 siRNA, Gaq or Gai minigene and in cells treated with pertussis toxin, and augmented by expression of dominant negative regulator of G protein signaling (RGS4(N88S)). Stimulation of Rho kinase activity was abolished by PAR-2 or Ga13 siRNA, and by Ga13 minigene. PAR2-AP induced a biphasic contraction; initial contraction was selectively blocked by the inhibitor of PI hydrolysis (U73122) or MLC kinase (ML-9), whereas sustained contraction was selectively blocked by the Rho kinase inhibitor (Y27632). PAR2-AP induced phosphorylation of MLC20, MYPT1 but not CPI-17. PAR2-AP also caused a decrease in the association of NF-kB and PKA catalytic subunit: the effect of PAR2-AP was blocked by PAR2 siRNA or phosphorylation-deficient RhoA (RhoA(S188A)). PAR2-AP-induced degradation of IkBa and activation of NF-kB were abolished by the blockade of RhoA activity by Clostridium botulinum C3 exoenzyme suggesting RhoA-dependent activation of NF-kB. PAR2-AP-stimulated Rho kinase activity was significantly augmented by the inhibitors of PKA (myristoylated PKI), IKK2 (IKKIV) or NF-kB (MG132), and in cells expressing dominant negative mutants of IKK (IKK(K44A), IkBa (IkBa (S32A/S36A)) or RhoA(S188A), suggesting feedback inhibition of Rho kinase activity via PKA derived from NF-kB pathway. PAR2-AP induced phosphorylation of RhoA and the phosphorylation was attenuated in cells expressing phosphorylation-deficient RhoA(S188A). Our results identified signaling pathways activated by PAR2 to mediate smooth muscle contraction and a novel pathway for feedback inhibition of PAR2-stimulated RhoA. The pathway involves activation of the NF-kB to release catalytic subunit of PKA from its binding to IkBa and phosphorylation of RhoA at Ser(188).
我们检测了蛋白酶激活受体2(PAR2)的表达,并对其在兔胃肌细胞中的信号通路进行了表征。PAR2激活肽SLIGRL(PAR2-AP)刺激Gq、G13、Gi1、磷脂酰肌醇(PI)水解和Rho激酶活性,并抑制环磷酸腺苷(cAMP)的形成。在表达PAR2小干扰RNA(siRNA)、Gaq或Gai小基因的细胞以及用百日咳毒素处理的细胞中,PI水解的刺激受到部分抑制,而通过表达G蛋白信号负调控因子(RGS4(N88S))可增强该刺激。PAR2或Gα13 siRNA以及Gα13小基因可消除Rho激酶活性的刺激。PAR2-AP诱导双相收缩;初始收缩被PI水解抑制剂(U73122)或肌球蛋白轻链激酶(MLC激酶,ML-9)选择性阻断,而持续收缩被Rho激酶抑制剂(Y27632)选择性阻断。PAR2-AP诱导肌球蛋白轻链20(MLC20)、肌球蛋白磷酸酶靶向亚基1(MYPT1)而非CPI-17的磷酸化。PAR2-AP还导致核因子κB(NF-κB)与蛋白激酶A(PKA)催化亚基的结合减少:PAR2-AP的作用被PAR2 siRNA或磷酸化缺陷型RhoA(RhoA(S188A))阻断。肉毒杆菌C3外切酶对RhoA活性的阻断消除了PAR2-AP诱导的IkBa降解和NF-κB激活,提示RhoA依赖的NF-κB激活。PKA抑制剂(肉豆蔻酰化PKI)、IKK2(IKKIV)或NF-κB(MG132)以及在表达IKK(IKK(K44A))、IkBa(IkBa(S32A/S36A))或RhoA(S188A)显性负突变体的细胞中,PAR2-AP刺激的Rho激酶活性显著增强,提示通过源自NF-κB途径的PKA对Rho激酶活性进行反馈抑制。PAR2-AP诱导RhoA磷酸化,在表达磷酸化缺陷型RhoA(S188A)的细胞中该磷酸化减弱。我们的结果确定了PAR2激活的介导平滑肌收缩的信号通路以及PAR2刺激的RhoA反馈抑制的新途径。该途径涉及NF-κB的激活,以从其与IkBa的结合中释放PKA催化亚基,并使RhoA在Ser(188)处磷酸化。
Zotero 插件