Increased endothelin receptor B and G protein coupled kinase-2 in the mesentery of portal hypertensive rats

AIM: To elucidate the mechanisms of mesenteric vasodilation in portal hypertension (PHT), with a focus on endothelin signaling. METHODS: PHT was induced in rats by common bile duct ligation (CBDL). Portal pressure (PP) was measured directly via catheters placed in the portal vein tract. The level of endothelin-1 (ET-1) in the mesenteric circulation was determined by radioimmunoassay, and the expression of the endothelin A receptor (ETAR) and endothelin B receptor (ETBR) was assessed by immunofluorescence and Western blot. Additionally, expression of G protein coupled kinase-2 (GRK2) and β-arrestin 2, which influence endothelin receptor sensitivity, were also studied by Western blot. RESULTS: PP of CBDL rats increased significantly (11.89 ± 1.38 mmHg vs 16.34 ± 1.63 mmHg). ET-1 expression decreased in the mesenteric circulation 2 and 4 wk after CBDL. ET-1 levels in the systemic circulation of CBDL rats were increased at 2 wk and decreased at 4 wk. There was no change in ETAR expression in response to CBDL; however, increased expression of ETBR in the endothelial cells of mesenteric arterioles and capillaries was observed. In sham-operated rats, ETBR was mainly expressed in the CD31+ endothelial cells of the arterioles. With development of PHT, in addition to the endothelial cells, ETBR expression was noticeably detectable in the SMA+ smooth muscle cells of arterioles and in the CD31+ capillaries. Following CBDL, increased expression of GRK2 was also found in mesenteric tissue, though there was no change in the level of β-arrestin 2. CONCLUSION: Decreased levels of ET-1 and increased ETBR expression in the mesenteric circulation following CBDL in rats may underlie mesenteric vasodilation in individuals with PHT. Mechanistically, increased GRK2 expression may lead to desensitization of ETAR, as well as other vasoconstrictors, promoting this vasodilatory effect.

Mechanisms of regulation and function of G-protein-coupled receptor kinases

G-protein-coupled receptor kinases (GRKs) interact with the agonist-activated form of G-protein-coupled receptor (GPCR) to affect receptor phosphorylation and to initiate profound impairment of receptor signaling, or desensitization. GPCR forms the largest family of cell surface receptors, and defects in GRK function have the potential consequence to affect GPCR-stimulated biological responses in many pathological situations.

MicroRNA-760 acts as a tumor suppressor in gastric cancer development via inhibiting G-protein-coupled receptor kinase interacting protein-1 transcription

BACKGROUND Gastric cancer(GC)has become a serious threat to people's health.Accumulative evidence reveals that dysregulation of numerous microRNAs(miRNAs)has been found during malignant formation.So far,the role of microRNA-760(miR-760)in the development of GC is largely unknown.AIM To measure the expression level of miR-760 in GC and investigate its role in gastric tumorigenesis.METHODS Real-time quantitative polymerase chain reaction and Western blot analysis were used to measure the expression of miR-760 and G-protein-coupled receptor kinase interacting protein-1(GIT1).Cell growth was detected by 3-(4,5-dimethyl-2-thiazolyl)-2,5-diphenyl-2-H-tetrazolium bromide(MTT)and cell colony formation assays.Apoptosis was assessed by flow cytometric analysis.The relationship between miR-760 and GIT1 was verified by luciferase reporter assay.RESULTS The results showed that the expression of miR-760 was decreased in GC and associated with poor clinical outcomes in GC patients.Furthermore,miR-760 restrained cell proliferation and cell colony formation and induced apoptosis in GC cells.In addition,miR-760 directly targeted GIT1 and negatively regulated its expression in GC.GIT1 was upregulated in GC and predicted a worse prognosis in GC patients.We also found that upregulation of GIT1 weakened the inhibitory CONCLUSION In conclusion,miR-760 targets GIT1 to inhibit cell growth and promote apoptosis in GC cells.Our data demonstrate that miR-760 may be a potential target for the treatment of GC.

Isoleucine, an Essential Amino Acid, Induces the Expression of Human <i>β</i>Defensin 2 through the Activation of the G-Protein Coupled Receptor-ERK Pathway in the Intestinal Epithelia

Anti-microbial peptides are essential for the intestinal innate immunity that protects the intestinal epithelia from attacks by foreign pathogens. Human β-defensin (HBD) is one of the pivotal anti-microbial peptides that are expressed in the colonic epithelia. This study investigated the effect and the signaling mechanism of inducible β-defensin HBD2 by an essential amino acid, isoleucine (Ile) in colonic epithelial cells. Here we examined the expression level of HBD2 on induction of Ile in epithelial cells, and checked this pathway. HBD2 mRNA was induced by co-incubation with IL-1α and Ile in Caco2 cells, but not by Ile alone. An inhibitor of either ERK or Gi, a subunit of G-proteins, reduced the induction of HBD2 mRNA by Ile. The treatment with Ile also increased the intracellular calcium ion concentration, thus suggesting that the GPCR and ERK signaling pathway mediate the effects of Ile. These results indicate that an essential amino acid, Ile, enhances the expression of an inducible β-defensin, namely HBD2, by IL-1α through the activation of GPCRs and ERK signaling pathway. The administration of Ile may therefore represent a possible option to safely treat intestinal inflammation.

Functionally diverse ligands modulate different activation states of the formyl peptide receptor 2,a G protein-coupled receptor

OBJECTIVE To identify the mechanisms by which the formyl peptide receptor 2(FPR2)mediates both inflammatory and anti-inflammatory signaling in an agonist-dependent manner.METHODS Cells expressing FPR2 were incubated with weak agonists,Aβ42 and Ac2-26,before stimulation with a strong agonist,WKYMVm.Calcium mobilization,c AMP inhibition and MAP kinase activation were measured.Intramolecular FRET were determined using FPR2 constructs with an ECFP attached to the C-terminus and a Fl As H binding motif embedded in the first or third intracellular loop(IL1 or IL3,respectively).RESULTS Aβ42 did not induce significant Ca^(2+) mobilization,but positively modulated WKYMVm-induced Ca^(2+) mobilization and c AMP reduction in a dose-variable manner within a narrow range of ligand concentrations.Treating FPR2-expressing cells with Ac2-26,a peptide with anti-inflammatory activity,negatively modulated WKYMVm-induced Ca^(2+) mobilization and c AMP reduction.Intramolecular FRET assay showed that stimulation of the receptor constructs with Aβ42 brought the C-terminal domain closer to IL1 but away from IL3.An opposite conformational change was induced by Ac2-26.The FPR2 conformation induced by Aβ42 corresponded to enhanced ERK phosphorylation and attenuated p38 MAPK phosphorylation,whereas Ac2-26 induced FPR2 conformational change corresponding to elevated p38 MAPK phosphorylation and reduced ERK phosphorylation.CONCLUSION Aβ42 and Ac2-26 induce different conformational changes in FPR2.These findings provide a structural basis for FPR2 mediation of inflammatory vs anti-inflammatory functions and identify a type of receptor modulation that differs from the classic positive and negative allosteric modulation.

肺癌患者GASP-1、LCN2和TPX2的表达水平及其与TNM分期和预后的相关性分析

目的探究肺癌患者血清G蛋白偶联受体相关分选蛋白1(GASP-1)、脂质运载蛋白-2(LCN2)、Xklp2靶蛋白(TPX2)表达水平及其与TNM分期和预后的相关性。方法选取2019年4月至2022年5月在南部战区总医院接受诊疗的92例肺癌患者作为观察组,同期选取92例健康体检者作为对照组。采集所有研究对象的外周静脉血样,检测血清GASP-1、LCN2、TPX2表达水平。将观察组按预后情况分为预后良好组和预后不佳组,比较2组患者血清GASP-1、LCN2、TPX2表达水平。分析肺癌患者血清GASP-1、LCN2、TPX2表达水平与TNM分期和预后的相关性。结果观察组血清GASP-1、LCN2、TPX2表达水平高于对照组(P<0.05);观察组TNM分期为Ⅲ、Ⅳ期的肺癌患者血清GASP-1、LCN2、TPX2表达水平高于TNM分期为Ⅰ、Ⅱ期的肺癌患者(P<0.05),TNM分期为Ⅳ期的患者血清GASP-1、LCN2、TPX2表达水平均高于TNM分期为Ⅲ期的患者(P<0.05)。预后良好组血清GASP-1、LCN2、TPX2水平均低于预后不佳组(P<0.05);观察组治疗前血清GASP-1、LCN2、TPX2表达水平均与TNM分期呈正相关(P<0.05),治疗后血清GASP-1、LCN2、TPX2表达水平均与预后呈负相关(P<0.05)。结论血清GASP-1、LCN2、TPX2表达水平与肺癌患者的TNM分期相关,在对症治疗后检测上述血清指标,可在一定程度上反映患者预后情况,为临床提供参考。

Desensitization of G-protein-coupled receptors induces vascular hypocontractility in response to norepinephrine in the mesenteric arteries of cirrhotic patients and rats

BACKGROUND: The increased β-arrestin-2 and its combination with G-protein-coupled receptors (GPCRs) lead to GPCRs desensitization. The latter may be responsible for decreased contractile reactivity in the mesenteric arteries of cirrhotic patients and rats. The present study is to investigate the machinery changes of α-adrenergic receptors and G proteins and their roles in the contractility of mesenteric arteries of cirrhotic patients and animal models. METHODS: Patients with cirrhosis due to hepatitis B and cirrhotic rats induced by CCl 4 were studied. Mesenteric artery contractility in response to norepinephrine was determined by a vessel perfusion system. The contractile effect of G protein-coupled receptor kinase-2 (GRK-2) inhibitor on the mesenteric artery was evaluated. The protein expression of the α 1 adrenergic receptor, G proteins, β-arrestin-2, GRK-2 as well as the activity of Rho associated coiled-coil forming protein kinase-1 (ROCK-1) were measured by Western blot. In addition, the interaction of α 1 adrenergic receptor with β-arrestin-2 was assessed by co-immunoprecipitation. RESULTS: The portal vein pressure of cirrhotic patients and rats was significantly higher than that of controls. The doseresponse curve to norepinephrine in mesenteric arteriole was shifted to the right, and EC 50 was significantly increased in cirrhotic patients and rats. There were no significant differences in the expressions of the α 1 adrenergic receptor and G proteins in the cirrhotic group compared with the controls. However, the protein expressions of GRK-2 and β-arrestin-2 were significantly elevated in cirrhotic patients and rats compared with those of the controls. The interaction of the α 1 adrenergic receptor and β-arrestin-2 was significantly aggravated. This interaction was significantly reversed by GRK-2 inhibitor. Both the protein expression and activity of ROCK-1 were significantly decreased in the mesenteric artery in patients with cirrhosis compared with those of the controls, and this phenomenon was not shown in the cirrhotic rats. Norepinephrine significantly increased the activity of ROCK-1 in normal rats but not in cirrhotic ones. Norepinephrine significantly increased ROCK-1 activity in cirrhotic rats when GRK-2 inhibitor was used. CONCLUSIONS: β-arrestin-2 expression and its interaction with GPCRs are significantly upregulated in the mesenteric arteries in patients and rats with cirrhosis. These upregulations result in GPCR desensitization, G-protein dysfunction and ROCK inhibition. These may explain the decreased contractility of the mesenteric artery in response to vasoconstrictors.

肝星状细胞特异性Grk2基因敲除小鼠模型的制备及鉴定

目的利用Cre-loxP基因敲除技术建立肝星状细胞特异性G蛋白偶联受体激酶2(G protein-coupled receptor kinase 2,GRK2)基因敲除小鼠模型,为研究GRK2在肝星状细胞中的生物学功能提供动物模型基础。方法将loxP标记的Grk2基因小鼠(Grk2^(fl/fl))和Lrat-Cre工具鼠进行多次繁殖,建立肝星状细胞特异性Grk2基因敲除(Grk2^(ΔHSC))小鼠模型。观察和分析小鼠的生长繁殖情况;通过PCR反应鉴定flox和Cre基因型;免疫荧光双染检测肝星状细胞中GRK2表达;Western blot检测小鼠肝星状细胞及肺、脾、肾脏、心脏组织中GRK2蛋白表达;HE染色观察肝脏及肺、脾、心脏、肾脏组织学形态。结果成功鉴定Grk2^(ΔHSC)小鼠基因型;两组小鼠体质量、繁殖能力无明显差异;免疫荧光双染及Western blot结果表明,Grk2^(ΔHSC)小鼠的肝星状细胞中GRK2蛋白水平明显低于对照组小鼠,Grk2^(ΔHSC)小鼠肺、脾、肾脏和心脏组织中GRK2蛋白表达与对照组相比无明显变化;HE染色结果显示,Grk2^(ΔHSC)小鼠肝脏及主要组织结构与Grk2^(fl/fl)相比差异无显著性,可用于后续研究。结论本研究应用Cre-loxP技术成功构建了肝星状细胞特异性Grk2基因敲除小鼠,为进一步研究GRK2在肝脏中的作用提供了优良工具。

雌激素受体GPR30通过TXNIP/NLRP3信号通路减弱氧糖剥夺/复氧诱导的BV-2细胞氧化应激损伤和炎症反应

目的:通过研究雌激素受体G蛋白偶联受体30(G protein-coupled receptor 30,GPR30)对氧糖剥夺/再灌注(oxygenglucose deprivation and reperfusion,OGD/R)BV-2小胶质细胞的氧化应激损伤和炎症反应的调控作用,探讨其对OGD/R BV-2小胶质细胞的保护作用及其相关机制。方法:取BV-2小胶质细胞ODG 4 h后再灌注2、4、6或12 h。Western blot检测细胞中GPR30的蛋白表达水平。将pcDNA3.1、pcDNA3.1-GPR30、sh-NC、sh-GPR30质粒转染BV-2小胶质细胞,OGD 4 h后再灌注12 h。qRT-PCR检测GPR30 mRNA的表达水平,验证其转染效率,Western blot检测细胞中GPR30、硫氧还蛋白相互作用蛋白(thioredoxin-interactingprotein,TXNIP)、NOD样受体热蛋白结构域相关蛋白3(NOD-like receptor thermal protein domain associated protein 3,NLRP3)、半胱氨酸天冬氨酸蛋白水解酶剪切体-1(cleaved cysteinyl aspartate specific proteinase-1,cleaved Caspase-1)的蛋白表达水平,ELISA检测细胞中活性氧(reactive oxygen species,ROS)、丙二醛(malondialdehyde,MDA)、超氧化物歧化酶(superoxide dismutase,SOD)、肿瘤坏死因子-α(tumor necrosis factor-α,TNF-α)、白细胞介素-6(interleukin-6,IL-6)、白细胞介素-1β(interleukin-1β,IL-1β)、白细胞介素-18(interleukin-18,IL-18)水平。结果:GPR30在OGD/R后显著上升,在6 h时达到峰值,而在12 h时与对照组没有显著差异。随后确定OGD处理4 h,复氧12 h的时间点进行后续实验。qRT-PCR验证慢病毒转染成功,与对照组相比,OGD/R组细胞中ROS、MDA、TNF-α、IL-6、IL-1β、IL-18水平及TXNIP、NLRP3、cleavedCaspase-1蛋白表达水平显著上升,SOD活性显著下降(P<0.05);过表达GPR30抑制了ROS、MDA、TNF-α、IL-6、IL-1β、IL-18水平及TXNIP、NLRP3、cleaved-Caspase-1蛋白表达水平,促进了SOD活性;而干扰GPR30表达发挥了相反的作用。结论:GPR30能抑制ODG/R处理后BV-2细胞内TXNIP/NLRP3信号通路分子的表达,抑制ODG/R诱导的BV-2细胞氧化应激损伤和炎症反应,这可能是其保护ODG/R细胞的分子机制之一。

Association of hepatocyte-derived growth factor receptor/caudal type homeobox 2 co-expression with mucosal regeneration in active ulcerative colitis

AIM:To characterize the regeneration-associated stem cell-related phenotype of hepatocyte-derived growth factor receptor(HGFR)-expressing cells in active ulcerative colitis(UC).METHODS:On the whole 38 peripheral blood samples and 38 colonic biopsy samples from 18 patients with histologically proven active UC and 20 healthy control subjects were collected.After preparing tissue microarrays and blood smears HGFR,caudal type homeobox 2(CDX2),prominin-1(CD133) and Musashi-1conventional and double fluorescent immunolabelings were performed.Immunostained samples were digitalized using high-resolution Mirax Desk instrument,and analyzed with the Mirax TMA Module software.For semiquantitative counting of immunopositive lamina propria(LP) cells 5 fields of view were counted at magnification x 200 in each sample core,then mean ± SD were determined.In case of peripheral blood smears,30 fields of view with 100 μm diameter were evaluated in every sample and the number of immunopositive cells(mean ± SD) was determined.Using 337 nm UVA Laser MicroDissection system at least 5000 subepithelial cells from the lamina propria were collected.Gene expression analysis of HGFR,CDX2,CD133,leucine-rich repeat-containing G-protein coupled receptor 5(Lgr5),Musashi-1 and cytokeratin20(CK20) were performed in both laser-microdisscted samples and blood samples by using real time reverse transcription polymerase chain reaction(RT-PCR).RESULTS:By performing conventional and double fluorescent immunolabelings confirmed by RT-PCR,higher number of HGFR(blood:6.7 ± 1.22 vs 38.5 ±3.18;LP:2.25 ± 0.85 vs 9.22 ± 0.65;P < 0.05),CDX2(blood:0 vs 0.94 ± 0.64;LP:0.75 ± 0.55 vs 2.11± 0.75;P < 0.05),CD133(blood:1.1 ± 0.72 vs 8.3± 1.08;LP:11.1 ± 0.85 vs 26.28 ± 1.71;P < 0.05)and Musashi-1(blood and LP:0 vs scattered) positive cells were detected in blood and lamina propria of UC samples as compared to controls.HGFR/CDX2(blood:0 vs 1± 0.59;LP:0.8 ± 0.69 vs 2.06 ± 0.72,P < 0.05)and Musashi-1/CDX2(blood and LP:0 vs scattered) coexpressions were found in blood and lamina propria of UC samples.HGFR/CD133 and CD133/CDX2 coexpressions appeared only in UC lamina propria samples.CDX2,Lgr5 and Musashi-1 expressions in UC blood samples were not accompanied by CK20 mRNA expression.CONCLUSION:In active UC,a portion of circulating HGFR-expressing cells are committed to the epithelial lineage,and may participate in mucosal regeneration by undergoing mesenchymal-to-epithelial transition.

Activation of β_2-Adrenergic Receptor Induced by Three Catecholamine Agonists:a Docking and Molecular Dynamics Study

We studied the activation of β2-adrenergic receptor（β2AR） by norepinephrine, epinephrine and isoprote- renol using docking and molecular dynamics（MD） simulation. The simulation was done on the assumption that β2AR was surrounded with explicit water and infinite lipid bilayer membrane at body temperature. So the result should be close to that under the physiological conditions. We calculated the structure of binding sites in β2AR for the three ac- tivators. We also simulated the change of the conformation ofβ2AR in the transmembrane regions（TMs）, in the mo- lecular switches, and in the conserved DRY（Aspartic acid, Arginine and Tyrosine） motif. This study provides detailed information concerning the structure ofβ2AR during activation process.

肺组织β-AR和GRK2与重症急性胰腺炎肺损伤的关系以及甲强龙的影响

目的:探讨重症急性胰腺炎(SAP)致急性肺损伤(ALI)大鼠肺组织β-AR和G蛋白偶联受体激酶2(GRK2)的变化规律以及甲强龙的影响。方法:SD大鼠36只,随机分为3组,每组12只。对照组,仅做十二指肠翻动;模型组,胰胆管逆行注射5%牛磺胆酸钠(1 mL/kg),建立SAP模型;干预组,建立SAP模型后1 h给予甲强龙(30 mg/kg)。于6 h和12 h分别处死大鼠6只取肺组织,放射配基结合实验测量肺组织β-AR最大结合容量Bmax和平衡解离常数Kd,免疫荧光法检测肺组织GRK2表达。结果:模型组和干预组胰腺组织损伤评分显著高于对照组,模型制备成功;模型组和干预组肺组织损伤评分显著高于对照组,发生SAP肺损伤;模型组β-AR Bmax显著低于对照组和干预组,Kd显著高于对照组和干预组;模型组GRK2的表达显著高于对照组和干预组。结论:SD大鼠肺组织有丰富的GRK2表达,SAP肺损伤大鼠肺组织GRK2表达显著增加,这可能是β-AR下调的重要机制。

GIT1通过BMP-2/p-Smad1/5/8信号通路调节骨折愈合

目的 :探讨G蛋白偶联受体激酶结合蛋白1(G-protein coupled receptor kinase-interacting protein 1,GIT1)影响骨折愈合的具体机制。方法:分别取GIT1基因敲除小鼠和同窝野生型小鼠制作股骨骨折模型,每组30只。造模成功后2周,免疫组化检测骨痂区软骨细胞矿化及p-Smad1/5/8表达量。分别取2组小鼠的骨髓间充质干细胞(bone marrow mesenchymal stem cells,BMSCs),予以10 ng/m L的骨形态发生蛋白2(bone morphogenetic protein 2,BMP2)刺激后检测Smad1/5/8磷酸化水平和核转入能力;取C3H10T1/2细胞,分别用1μg p GL3重组质粒和1μg GIT1-si RNA共转染细胞,荧光报告素酶技术检测细胞内GIT1蛋白对BMP2转录水平的影响。结果:与同窝野生型小鼠相比,GIT1基因敲除小鼠软骨内骨化减弱,骨痂区软骨细胞堆积,骨折愈合延迟,p-Samd1/5/8表达水平明显减少;与GIT1基因敲除小鼠相比,BMP2可明显提高同窝野生型小鼠BMCs中p-Samd1/5/8核转入能力;GIT1蛋白表达的缺失可明显降低BMP2的转录水平。结论 :GIT1可通过调节Samd1/5/8的磷酸化及BMP2信号转导影响骨折部位的软骨内骨化。

运动上调GPR48-RANKL通路影响2型糖尿病小鼠破骨细胞分化

目的:探究T2DM小鼠OC分化变化及不同力学刺激通过GPR48-RANKL通路对T2DM小鼠OC分化的分子调控作用。方法:40只4周龄雄性C57BL/6小鼠,适应性喂养1周后随机分为T2DM造模组(30只)和正常对照组(ZC,10只)。T2DM造模组小鼠6周高脂膳食结束空腹12 h后注射STZ,2周后检测小鼠血糖,有27只造模成功并将其随机分为T2DM对照组(TC,9只)、T2DM游泳组(TS,9只)和T2DM游泳组(TD,9只),TS和TD组小鼠分别进行8周游泳和下坡跑训练。结束后,取右侧股骨并利用RT-PCR法检测相关因子mRNA表达;取左侧胫骨并利用West-blotting法检测相关因子蛋白表达;取小鼠BMM并诱导其向OC分化,利用TRAP染液对OC染色;取右侧胫骨并利用游标卡尺检测其大小。结果:与ZC组相比,TC组GPR48、OPG、RANKL、RANK、NFATc2、CTSK的mRNA和GPR48、RANKL、RANK蛋白表达均显著变化(P<0.05或P<0.01),OC数量显著增多,远端冠状面宽度和近端冠状面宽度显著变小(P<0.05)。与TC组相比,TS组GPR48、OPG、RANKL、NFATc2、CTSKmRNA和GPR48、RANKL蛋白表达均显著变化(P<0.05或P<0.01),OC数量显著减少;TD组GPR48、OPG、RANKL、RANK、NFATc2、CTSKmRNA和GPR48、RANKL、RANK蛋白表达均显著上调(P<0.05或P<0.01),OC数量显著减少,胫骨长度和中间矢状轴宽度显著减少(P<0.05或P<0.01)。与TS组相比,TD组OPG和CTSKmRNA及GPR48、RANK、RANKL蛋白表达均显著变化(P<0.05或P<0.01),OC数量显著减少。结论:T2DM小鼠OC分化显著增强;直接作用力激活T2DM小鼠骨中GPR48-RANKL通路,进而抑制RANK及其下游靶基因表达,抑制OC分化,且其作用效果优于间接作用力。

GIT1-WT及GIT1-Y293F慢病毒载体的构建及其对成骨细胞迁移能力的影响

目的:设计构建G蛋白偶联受体激酶结合蛋白1(G protein coupled receptor kinase interacting protein 1,GIT1)野生型(WT)及点突变型(Y293F)慢病毒载体,探讨293位点对GIT1功能的影响。方法:用PCR从小鼠cDNA文库中扩增GIT1-WT,将其连接到慢病毒载体PLJM-GFP中,构建质粒PLJM-GFP-GIT1-WT,测序鉴定。利用TaKaRa MutanBEST Kit试剂盒,对PLJM-GFP-GIT1-WT进行定点突变,构建质粒PLJM-GFP-GIT1-Y293F,测序鉴定。重组慢病毒载体转染包装细胞293T,获取病毒上清感染培养至第4代的小鼠成骨细胞。划痕愈合试验检测成骨细胞迁移能力的变化。结果:通过PCR鉴定、双酶切鉴定及测序鉴定,成功构建了PLJM-GFP-GIT1-WT与PLJM-GFP-GIT1-Y293F。划痕愈合试验观察,与PLJM-GFP-GIT1-WT相比,PLJM-GFP-GIT1-Y293F明显抑制成骨细胞迁移。结论:GIT1功能的正常发挥有赖于293位点适时的磷酸化。

人源GRK2的真核表达、纯化及活性检测

目的构建人源G蛋白偶联受体激酶2(GRK2)真核表达系统。方法设计引物,以pIRES-EGFP-GRK2(全长)基因为模板,PCR扩增His-GRK2目的基因,将His-GRK2目的基因连接在pcDNA3.1-EGFP真核表达载体上;将pcDNA3.1-EGFP-His-GRK2质粒转染至HEK 293T细胞,48 h后采用Western blot法检测GRK2蛋白表达,通过镍螯合的磁珠法纯化GRK2蛋白,考马斯亮蓝染色和Western blot法检测GRK2蛋白纯化,His pull down检测GRK2蛋白活性。结果双酶切和测序鉴定结果表明,pcDNA3.1-EGFP-His-GRK2真核表达质粒成功构建;Western blot法检测结果表明,GRK2蛋白的分子量约为80 ku,提示GRK2蛋白在HEK 293T细胞中成功表达(t=6.433,P=0.003);通过镍螯合的磁珠纯化得到GRK2蛋白,His pull down实验结果表明GRK2与前列腺素E2受体4亚型(EP4)结合,提示GRK2蛋白具有生物学活性(t=13.5,P=0.0002)。结论pcDNA3.1-EGFP-His-GRK2真核表达质粒的序列测序正确,成功构建GRK2重组质粒,GRK2重组质粒在真核细胞HEK 293T的细胞中成功表达且表达的蛋白具有生物学活性。

诱导型巨噬细胞特异性敲除GRK2基因小鼠模型的构建及应用

目的 建立诱导型巨噬细胞特异性敲除G蛋白偶联受体激酶2(GRK2)基因(GRK2^(flox/flox)Lyz2-CreERT^(+))小鼠模型。方法 基于Cre/LoxP系统构建GRK2^(flox/flox)Lyz2-CreERT^(+)小鼠。通过PCR扩增程序及琼脂糖凝胶电泳鉴定GRK2^(flox/flox)Lyz2-CreERT^(+)小鼠的基因型。二氧化碳法处死小鼠后,Western blot检测骨髓源巨噬细胞(BMDMs)和腹腔巨噬细胞(PMs)中GRK2表达。免疫荧光检测小鼠脑、心脏和脾脏巨噬细胞中GRK2表达。流式细胞术分析前列腺素E2(PGE2)诱导的PMs中M1/M2比例。结果 基因型鉴定结果表明,flox扩增产物长度在355 bp处有一条条带且Cre扩增产物长度在355 bp处有一条条带的小鼠即为GRK2^(flox/flox)Lyz2-CreERT^(+)小鼠。Western blot结果显示,与GRK2^(flox/flox)小鼠相比,GRK2^(flox/flox)Lyz2-CreERT^(+)小鼠BMDMs和PMs中GRK2表达降低(P<0.01)。免疫荧光结果显示,与GRK2^(flox/flox)小鼠相比,GRK2^(flox/flox)Lyz2-CreERT^(+)小鼠脑、心脏和脾脏中GRK2表达降低(P<0.01)。流式细胞术结果显示,与GRK2^(flox/flox)小鼠相比,GRK2^(flox/flox)Lyz2-CreERT^(+)小鼠PMs中CD86/CD206比例变化差异无统计学意义。在PGE2(10μmol/L)刺激下,GRK2^(flox/flox)Lyz2-CreERT^(+)小鼠PMs中CD86/CD206比例升高(P<0.01),且GRK2^(flox/flox)小鼠PMs中CD86/CD206比例高于GRK2^(flox/flox)Lyz2-CreERT^(+)小鼠(P<0.01)。结论 该研究成功构建出GRK2^(flox/flox)Lyz2-CreERT^(+)小鼠模型,且该小鼠可促进PGE2诱导的PMs向M2型巨噬细胞极化。

G蛋白耦联受体激酶2在MPTP诱导的PD模型小鼠纹状体中的作用机制

目的 探究G蛋白耦联受体激酶(GRK)2在帕金森病(PD)小鼠纹状体中的作用机制。方法 选用C57BL/J雄性8周龄小鼠,随机分为对照组和模型组;对照组腹腔注射0.2 ml生理盐水,模型组腹腔注射30 mg/kg的1-甲基-4-苯基-1,2,3,6-四氢吡啶(MPTP),2次/w,共5 w。35 d后对两组进行爬杆实验和旷场实验检测。行为学检测后,小鼠麻醉后眼球取血、取脑,运用酶联免疫吸附试验(ELISA)及免疫组化检测血清和中脑酪氨酸羟化酶(TH)表达,Western印迹和免疫组化检测纹状体GRK2和多巴胺2受体(D2R)表达。结果 在旷场实验中,MPTP干预后模型组自发活动总距离、穿越中心格次数和距离比对照组明显减少(均P<0.001)。在爬杆实验中,模型组爬杆时间比对照组明显延长(P<0.001)。ELISA及免疫组化显示,模型组血清和中脑TH值较对照组明显减少(P<0.001)。Western印迹和免疫组化提示,与对照组相比,纹状体D2R表达显著减少,而CRK2表达显著升高(P<0.05)。结论 GRK2可能通过D2R参与调控PD的症状,针对GRK2是潜在的PD治疗靶点。

猪GRK2蛋白抗口蹄疫病毒作用分析

为研究G蛋白偶联受体激酶2(G protein-coupled receptor kinase 2,GRK2)对口蹄疫病毒(foot-and-mouth disease virus,FMDV)复制的影响,从猪的PK-15细胞中提取RNA,通过聚合酶链式反应(polymerase chain reaction,PCR)扩增出猪GRK2的完整CDS序列,并构建了猪GRK2真核表达质粒。Western blot和间接免疫荧光试验表明GRK2可表达并定位于细胞质中。FMDV感染PK-15细胞的GRK2转录水平和蛋白水平呈先上升后下降趋势;过表达GRK2可显著抑制FMDV的复制,下调表达GRK2可显著促进FMDV的复制,表明GRK2在FMDV感染过程中具有抗病毒作用。进一步研究发现FMDV 3C^(pro)蛋白可与GRK2互作并降解GRK2,促进FMDV的复制。研究结果为进一步分析宿主蛋白GRK2的抗FMDV的分子机制奠定了基础。

肠道菌群-胆汁酸途径对2型糖尿病的影响

目的综述肠道菌群-胆汁酸通路对2型糖尿病(T2DM)发生发展及防治的研究进展,为基于该通路的糖尿病防治提供文献参考,为开发治疗糖尿病的创新治疗方法提供思路。方法通过查阅国内外相关文献,我们综述了肠道菌群与T2DM的相关性、胆汁酸和T2DM相关性、肠道菌群与胆汁酸代谢的相关性,并重点论述了肠道菌群-胆汁酸通路在T2DM发生发展及防治中的研究进展,强调该路径对血糖调节方面的局限性和挑战,并探讨如何基于该路径开发防治T2DM的创新方法。结果与结论肠道菌群-胆汁酸通路可介导T2DM的发生发展。肠道菌群可通过一系列酶促反应,影响初级胆汁酸转变为次级胆汁酸,随后通过法尼醇X受体(FXR)、G蛋白偶联胆汁酸受体5(TGR5)调节信号传导,影响宿主的代谢途径。FXR和TGR5受体已成为糖尿病等代谢疾病研究的新靶点,开发肠道特异性FXR拮抗剂和TGR5激动剂可能是未来治疗T2DM的一个很有前途的方法,然而其长期效果值得进一步评估。