Buxu Tongyu Granule Alleviates Myocardial Ischemia by Activating Vascular Smooth Muscle Cell Soluble Guanylate Cyclase to Inhibit Abnormal Vasomotion

Myocardial ischemia is a serious threat to human health,and vascular dysfunction is its main cause.Buxu Tongyu(BXTY)Granule is an effective traditional Chinese medicine(TCM)for treating myocardial ischemia.However,the underlying mechanism of BXTY is still unclear.In this study,we demonstrate that BXTY ameliorates myocardial ischemia by activating the soluble guanylate cyclase(sGC)-30,50-cyclic guanosine monophosphate(cGMP)-protein kinase G(PKG)signaling pathway in vascular smooth muscle cells(VSMCs)to dilate the arteries.BXTY was given by gavage for ten consecutive days before establishing an animal model of acute myocardial ischemia in mice via the intraperitoneal injection of pituitrin.The results showed that BXTY alleviated the symptoms of myocardial ischemia induced by pituitrin in mice,including electrocardiogram abnormalities and changes in plasma enzymes.In addition,BXTY dilated pre-constricted blood vessels and inhibited the vasoconstriction of the superior mesenteric artery in a dose-dependent but endothelial-independent manner.These effects were eliminated by preincubating vascular rings with the sGC inhibitors NS 2028 or ODQ,or with the PKG inhibitor KT 5823.Moreover,BXTY increased the protein expression of sGC-b1 and the intracellular second messenger cGMP level in mouse aortic vascular smooth muscle cells(MOVAs).NS 2028 or ODQ reversed these effects of BXTY.The expression level of the cGMP downstream effector protein PKG-1 increased after treating MOVAs with BXTY.NS 2028,ODQ,or KT 5823 also reversed this effect of BXTY.In conclusion,BXTY can improve the symptoms of acute myocardial ischemia in mice,and activating the sGC-cGMP-PKG pathway in VSMCs to induce vasodilation is its key pharmacodynamic mechanism.

Safety and efficacy of soluble guanylate cyclase stimulators in patients with heart failure: A systematic review and meta-analysis

BACKGROUND The utility of novel oral soluble guanylate cyclase(sGC)stimulators(vericiguat and riociguat),in patients with reduced or preserved ejection fraction heart failure(HFrEF/HFpEF)is currently unclear.AIM To determine the efficacy and safety of sGC stimulators in HF patients.METHODS Multiple databases were searched to identify relevant randomized controlled trials(RCTs).Data on the safety and efficacy of sGC stimulators were compared using relative risk ratio(RR)on a random effect model.RESULTS Six RCTs,comprising 5604 patients(2801 in sGC stimulator group and 2803 placebo group)were included.The primary endpoint(a composite of cardiovascular mortality and first HF-related hospitalization)was significantly reduced in patients receiving sGC stimulators compared to placebo[RR 0.92,95%confidence interval(CI):0.85-0.99,P=0.02].The incidence of total HF-related hospitalizations were also lower in sGC group(RR 0.91,95%CI:0.86-0.96,P=0.0009),however,sGC stimulators had no impact on all-cause mortality(RR 0.96,95%CI:0.86-1.07,P=0.45)or cardiovascular mortality(RR 0.94,95%CI:0.83-1.06,P=0.29).The overall safety endpoint(a composite of hypotension and syncope)was also similar between the two groups(RR 1.50,95%CI:0.93-2.42,P=0.10).By contrast,a stratified subgroup analysis adjusted by type of sGC stimulator and HF(vericiguat vs riociguat and HFrEF vs HFpEF)showed near identical rates for all safety and efficacy endpoints between the two groups at a mean follow-up of 19 wk.For the primary composite endpoint,the number needed to treat was 35,the number needed to harm was 44.CONCLUSION The use of vericiguat and riociguat in conjunction with standard HF therapy,shows no benefit in terms of decreasing HF-related hospitalizations or mortality.

Plecanatide and dolcanatide, novel guanylate cyclase-C agonists, ameliorate gastrointestinal inflammation in experimental models of murine colitis

AIM: To evaluate the effect of orally administeredplecanatide or dolcanatide, analogs of uroguanylin, on amelioration of colitis in murine models.METHODS: The cyclic guanosine monophosphate(cG MP) stimulatory potency of plecanatide and dolcanatide was measured using a human colon carcinoma T84 cellbased assay. For animal studies all test agents were formulated in phosphate buffered saline. Sulfasalazine or 5-amino salicylic acid(5-ASA) served as positive controls. Effect of oral treatment with test agents on amelioration of acute colitis induced either by dextran sulfate sodium(DSS) in drinking water or by rectal instillation of trinitrobenzene sulfonic(TNBS) acid, was examined in BALB/c and/or BDF1 mice. Additionally, the effect of orally administered plecanatide on the spontaneous colitis in T-cell receptor alpha knockout(TCRα-/-) mice was also examined. Amelioration of colitis was assessed by monitoring severity of colitis, disease activity index and by histopathology. Frozen colon tissues were used to measure myeloperoxidase activity.RESULTS: Plecanatide and dolcanatide are structurally related analogs of uroguanylin, which is an endogenous ligand of guanylate cyclase-C(GC-C). As expected from the agonists of GC-C, both plecanatide and dolcanatide exhibited potent cG MP-stimulatory activity in T84 cells. Once-daily treatment by oral gavage with either of these analogs(0.05-0.5 mg/kg) ameliorated colitis in both DSS and TNBS-induced models of acute colitis, as assessed by body weight, reduction in colitis severity(P < 0.05) and disease activity index(P < 0.05). Amelioration of colitis by either of the drug candidates was comparable to that achieved by orally administered sulfasalazine or 5-ASA. Plecanatide also effectively ameliorated colitis in TCRα-/- mice, a model of spontaneous colitis. As dolcanatide exhibited higher resistance to proteolysis in simulated gastric and intestinal juices, it was selected for further studies. CONCLUSION: This is the first-ever study reporting the therapeutic utility of GC-C agonists as a new class of orally delivered and mucosally active drug candidates for the treatment of inflammatory bowel diseases.

Plecanatide-mediated activation of guanylate cyclase-C suppresses inflammation-induced colorectal carcinogenesis in Apc+/Min-FCCC mice

AIM To evaluate the effect of orally administered plecanatide on colorectal dysplasia in Apc^(+/Min-FCCC) mice with dextran sodium sulfate(DSS)-induced inflammation. METHODS Inflammation driven colorectal carcinogenesis was induced in Apc^(+/Min-FCCC) mice by administering DSS in their drinking water. Mice were fed a diet supplemented with plecanatide(0-20 ppm) and its effect on the multiplicity of histopathologically confirmed polypoid,flat and indeterminate dysplasia was evaluated. Plecanatide-mediated activation of guanylate cyclase-C(GC-C) signaling was assessed in colon tissues by measuring cyclic guanosine monophosphate(cG MP) by ELISA, protein kinase G-II and vasodilator stimulated phosphoprotein by immunoblotting. Ki-67, c-myc and cyclin D1 were used as markers of proliferation. Cellular levels and localization of b-catenin in colon tissues were assessed by immunoblotting and immunohistochemistry, respectively. Uroguanylin(UG) and GC-C transcript levels were measured by quantitative reverse transcription polymerase chain reaction(RT-PCR). A mouse cytokine array panel was used to detect cytokines in the supernatant of colon explant cultures. RESULTS Oral treatment of Apc^(+/Min-FCCC) mice with plecanatide produced a statistically significant reduction in the formation of inflammation-driven polypoid, flat and indeterminate dysplasias. This anti-carcinogenic activity of plecanatide was accompanied by activation of cG MP/GC-C signaling mediated inhibition of Wnt/b-catenin signaling and reduced proliferation. Plecanatide also decreased secretion of pro-inflammatory cytokines(IL-6, IL-1 TNF), chemokines(MIP-1, IP-10) and growth factors(GCSF and GMCSF) from colon explants derived from mice with acute DSS-induced inflammation. The effect of plecanatidemediated inhibition of inflammation/dysplasia on endogenous expression of UG and GC-C transcripts was measured in intestinal tissues. Although GC-C expression was not altered appreciably, a statistically significant increase in the level of UG transcripts was detected in the proximal small intestine and colon, potentially due to a reduction in intestinal inflammation and/or neoplasia. Taken together, these results suggest that reductions in endogenous UG, accompanied by dysregulation in GC-C signaling, may be an early event in inflammation-promoted colorectal neoplasia; an event that can potentially be ameliorated by prophylactic intervention with plecanatide.CONCLUSION This study provides the first evidence that orally administered plecanatide reduces the multiplicity of inflammation-driven colonic dysplasia in mice, demonstrating the utility for developing GC-C agonists as chemopreventive agents.

Isolation,Purification and Spectral Characteristics of Soluble Guanylate Cyclase from Bovine Lung

We isolated and purified high purity and high activity soluble Guanylate cyclase(sGC) from bovine lung. The electronic absorption and resonance Raman spectra of the ferrous and ferric forms of sGC were recorded. In the ferrous state of sGC, the electronic absorption spectra showed a sharp peak at 431 nm and a single broad peak in the α/β region at 559 nm. The resonance Raman spectra of sGC(ferrous) showed a stronger band at 1357 cm -1 and a single peak at 1473 cm -1 . For the ferric form of sGC, the Soret band was at 390 nm and resonance Raman peak was at 1375 cm -1 . These spectra show that the heme iron of the ferrous and ferric sGC are all 5 coordination and high spin.

长链非编码RNA GC1靶向微小RNA-551b-3p抑制食管癌的作用及分子机制研究

目的探讨长链非编码RNA(LncRNA)鸟苷酸环化酶1(GC1)对食管癌的影响,并探讨其靶向微小RNA-551b-3p(miR-551b-3p)的分子机制。方法建立食管癌荷瘤裸小鼠模型,随机分为GC1、miR-551b-3p上、下调组及其对应对照组与模型组共9组,每组8只。末次给药次日处死裸小鼠,称取瘤体质量,计算抑瘤率;取肿瘤组织检测LncRNA GC1、miR-551b-3p基因表达水平和细胞周期因子(CyclinD1)、p21、B淋巴细胞瘤-2(Bcl-2)、Bcl-2相关x(Bax)基因与蛋白表达水平;观察肿瘤组织病理改变;采用流式细胞术检测肿瘤细胞凋亡率;采用双荧光素酶报告基因实验验证LncRNA GC1与miR-551b-3p的调控关系。另取人食管癌细胞株Eca109分为9组,每组3个复孔,其中基因干扰组命名同上,另设置空白组,培养48h后观察细胞LncRNA GC1、miR-551b-3p基因表达水平、形态学改变、凋亡率、CyclinD1、p21、Bcl-2、Bax基因与蛋白表达水平。结果动物实验:与模型组和相应对照组比较,GC1上调组与miR-551b-3p下调组瘤体质量、CyclinD1和Bcl-2基因与蛋白表达水平均上升,抑瘤率、细胞凋亡率、miR-551b-3p基因、p21和Bax基因与蛋白表达水平均下降;GC1下调组与miR-551b-3p上调组瘤体质量、CyclinD1和Bcl-2基因与蛋白表达水平均下降,抑瘤率和细胞凋亡率、miR-551b-3p基因、p21和Bax基因与蛋白表达水平均上升;GC1上调组LncRNA GC1基因表达水平上升,GC1下调组LncRNA GC1基因表达水平下降(P<0.05)。与转染野生型GC1的腺病毒载体相比,转染突变型GC1的腺病毒载体的miR-551b-3p荧光素酶相对活性上升(P<0.05)。细胞实验:LncRNA GC1和miR-551b-3p基因表达水平、细胞形态学改变与凋亡率、CyclinD1、p21、Bcl-2、Bax基因与蛋白表达水平变化趋势均与动物实验相同。结论下调LncRNA GC1、上调miR-551b-3p表达水平均可抑制食管癌进展,且下调LncRNA GC1可靶向上调miR-551b-3p,并降低CyclinD1和Bcl-2活性、上升p21和Bax活性。

新型sGC刺激剂维立西呱在心衰治疗中的价值

目的:探讨新型可溶性鸟苷酸环化酶(sGC)刺激剂维立西呱在心衰(HF)治疗中的价值。方法:2022年10月~2023年6月本院收治的60例HF患者,随机数字表法分为维立西呱组和对照组,每组各30例。对照组采用常规抗HF治疗,维立西呱组在对照组基础上给予维立西呱口服,均持续3 m。比较两组的心功能改善疗效和治心室重构指标、心功能及不良反应发生率。结果:维立西呱组心功能改善疗效为93.33%,高于对照组的73.33%(P<0.05)。维立西呱组LVEF、6MWT高于对照组,LVESV、LVEDD和NT-ProBNP低于对照组(P<0.05)。结论:新型sGC刺激剂维立西呱治疗可改善HF患者心功能和运动耐力,降低NT-ProBNP水平。

青藤碱对吗啡依赖小鼠脊髓与小脑中HO2、sGCα1和sGCα2基因mRNA表达的影响

目的评价青藤碱治疗前后吗啡依赖与戒断小鼠脊髓和小脑中HO2、sGCα1和sGCα2基因mRNA水平的变化,探讨青藤碱作用于吗啡依赖小鼠的分子机制。方法采用吗啡剂量递增法,建立小鼠吗啡依赖模型,用青藤碱(40mg.kg-1,ip)治疗吗啡依赖小鼠后,再用纳洛酮激发急性戒断症状,半定量RT-PCR测脊髓和小脑HO2、sGCα1和sGCα2基因的mRNA水平变化。结果慢性吗啡用药使小鼠脊髓与小脑中HO2和sGCα1基因的mRNA水平发生异常上调,sGCα2基因的mRNA水平没有异常上调。单独使用青藤碱,没有引起小鼠脊髓与小脑中这些指标异常升高。青藤碱治疗后,小鼠吗啡依赖与戒断时在脊髓与小脑中异常上调的HO2和sGCα1基因的mRNA水平下降到接近对照组水平。结论慢性吗啡用药使HO2和sGCα1基因的mRNA水平发生不同程度的异常上调,这种上调在青藤碱治疗后可以恢复到接近正常水平,这可能是青藤碱对吗啡依赖小鼠治疗作用的分子机制之一。

慢性低O_2高CO_2时NO-sGC-cGMP细胞信号转导通路变化及与肺动脉高压的关系

目的 :探讨慢性低O2 高CO2 性肺动脉高压发生与发展中NO sGC cGMP细胞信号转导通路的变化和作用。方法 :雄性Sprague Dawley大鼠随机分为对照组与低O2 高CO2 肺动脉高压 1w、2w及 4w组。用比色法测定血浆NO含量 ,酶动力学法测定肺组织sGC活性 ,12 5 I 放射免疫法检测肺组织cGMP含量。结果 :低O2 高CO2 1w、2w、4w组mPAP较对照组均明显升高 (P均 <0 .0 1)。而血浆NO含量、肺组织sGC活性和肺组织cGMP含量均显著降低 (分别P <0 .0 5,P <0 .0 1或P <0 .0 0 1)。mPAP与血浆NO含量 (r =-0 .80 7,P <0 .0 1)、与肺组织sGC活性 (r=-0 .754,P <0 .0 1)、与肺组织cGMP含量 (r=-0 .62 1,P <0 .0 1)之间均存在显著负相关。结论 :低O2 高CO2 引起的NO sGC

shRNA抑制GC-C基因表达对人胃癌SGC-7901细胞生物学功能的影响

目的研究靶向鸟苷酸环化酶C(GC-C)的短发夹RNA(shRNA)对人胃癌SGC-7901细胞增殖、凋亡和细胞周期等生物学功能的影响。方法构建针对人GC-C基因的shRNA真核表达载体,将其转染入人胃癌SGC-7901细胞,采用半定量RT-PCR和Western blotting法检测细胞中GC-C在mRNA和蛋白水平的变化。以CCK-8法、流式细胞术和原位末端标记法检测转染GC-CshRNA真核表达载体的SGC-7901细胞增殖、凋亡及细胞周期等生物学指标的变化。结果经DNA测序鉴定,所得到的表达载体插入片段序列与GenBank中的序列一致。shRNA-GC-C真核表达载体转染能有效抑制GC-C基因的表达,以shRNA-GC-CⅢ序列的抑制效果最佳。转染GC-CshRNA真核表达载体后SGC-7901细胞的增殖能力受到抑制(P<0.05);细胞形态发生改变,细胞体积缩小,核固缩,染色质浓缩聚集于核膜;流式细胞术检测显示G1峰前出现亚二倍体峰,转染48、72h后凋亡率分别为5.47%和5.63%(P<0.05)。结论靶向GC-C基因的shRNA可有效抑制人胃癌SGC-7901细胞生长,并促进细胞凋亡,该作用与下调靶基因GC-C的表达有关;GC-C可能是胃癌治疗的一个潜在靶点。

姜黄素通过HO/GC途径对抗高糖诱导的血管收缩功能下降

目的:研究姜黄素是否可对抗高糖诱导的血管收缩功能下降,并探讨其作用机制。方法:采用血管环离体灌流装置,观察SD大鼠胸主动脉环的收缩反应;测定主动脉胆红素生成量反映血红素加氧酶-1(HO-1)的活性。结果:(1)与空白对照组(含11mmol/L葡萄糖)相比,经44mmol/L葡萄糖(高糖)孵育血管4h后,主动脉环对苯肾上腺素(PE)引起的血管收缩反应下降;(2)姜黄素(3×10-11-3×10-10mol/L)与高糖联合孵育,均能不同程度地抑制高糖诱导的血管PE收缩反应的下降;(3)姜黄素孵育后可引起血管HO活性增高;HO-1抑制剂锌原卟啉Ⅸ(ZnPP)可完全取消姜黄素的抗高糖损伤作用;(4)鸟苷酸环化酶(GC)抑制剂亚甲蓝可部分阻断姜黄素的保护作用。结论:姜黄素可能通过诱导HO-1活性增加和激活GC途径对抗高糖引起的血管收缩功能降低。

新型可溶性鸟苷酸环化酶激动剂sGC003对内皮素诱导的心肌细胞肥大的作用

目的研究可溶性鸟苷酸环化酶（s GC）激动剂s GC003对内皮素1（ET-1）诱导的心肌细胞肥大的作用。方法通过复合酶消化法及差速贴壁法培养SD乳大鼠原代心肌细胞,以ET-1 10 nmol·L-1刺激其发生肥大,同时给予s GC003 0.01,0.1和1.0μmol·L-1,48 h后在倒置显微镜下观察心肌细胞形态,图像分析软件（Image-Pro Plus6.0）对心肌细胞表面积进行测量分析,BCA法检测心肌细胞总蛋白质含量,实时定量PCR法检测心房利钠肽基因（ANP）m RNA表达。结果与正常对照组相比,ET-1 10 nmol·L-1刺激心肌细胞48 h,可使心肌细胞表面积增加80%（P〈0.01）,总蛋白质含量增加120%（P〈0.01）,ANP m RNA水平升高140%（P〈0.01）。给予s GC003 0.01～1.0μmol·L-1能对抗ET-1引起的心肌细胞表面积增大（P〈0.01）和总蛋白质含量升高（P〈0.05）,对于ET-1诱导的ANP m RNA表达增加也有一定抑制作用（P〈0.05）。结论s GC003可改善ET-1诱导的心肌细胞肥大,对心肌细胞具有保护作用。

GC-C^(-/-)小鼠在DSS诱导下肠道炎症损伤的变化

目的了解鸟苷酸环化酶C(GC-C)信号通路在右旋糖酐硫酸酯钠(DSS)诱导小鼠肠道炎症性损伤发生中的作用。方法运用DSS构建GC-C基因敲除(GC-C^(-/-))小鼠和野生型(WT)小鼠结肠炎模型,将小鼠分为炎症组和对照组,前者给予3%的DSS溶液自由饮用1周,后者给予正常饮食。运用qRT-PCR和Westernblot方法检测结肠组织GC-C mRNA和蛋白的表达,在光学显微镜下观察经HE染色后结肠组织的炎症损伤情况并进行组织病理学评分。运用ELISA方法检测小鼠外周血与肠黏液中炎症因子(IL-8和TNF-α)的水平。结果(1)与WT小鼠相比,GC-C^(-/-)小鼠在DSS作用下疾病活动指数(DAI)评分明显升高(P<0.05),结肠缩短、肠管增粗、充血水肿更明显;(2)显微镜下观察到GC-C^(-/-)+DSS组小鼠结肠组织炎症损伤更为严重,组织病理学评分较WT+DSS组小鼠明显升高(P<0.05);(3)GC-C^(-/-)小鼠在DSS诱导下外周血和肠粘液中IL-8和TNF-α水平较WT+DSS组明显升高(P<0.05)。结论GC-C^(-/-)小鼠在化学物质诱导下肠道炎症性损伤加重,GC-C信号通路可能参与了溃疡性结肠炎(UC)的发生与发展。

外周血GC-CmRNA的检测对大肠癌微转移的诊断价值

目的探讨外周血中鸟苷环化酶CmRNA(GCC-mRNA)的表达对大肠癌微转移的诊断意义。方法1、制备微转移模型;2、收集周围血标本:大肠癌患者67例,正常人及良性胃肠道疾病患者20例。3、检测GCC-mRNA:逆转录聚合酶链反应法检测GCC-mRNA。结果1、微转移模型:微转移模型GCC-mRNA表达阳性率为85%;对照组正常人外周血20例中无一例阳性;大肠癌微转移模型标本及对照组中的表达差异显著(P<0.001)。2、结肠癌:结肠癌GCC-mRNA表达阳性率为58%,良性胃肠道疾病为20%,正常人为0%,三组比较差异显著(P<0.01)。大肠癌患者有结肠外转移阳性率为72%;无转移阳性率为52%,二组差异无显著性(P>0.05)。3、GCC与CEA:GC-C与CEA总阳性率分别为58%与27%,前者显著高于后者(P<0.01)。结论1、提示RT-PCR法检测GC-C诊断大肠癌微转移方法有希望用于诊断大肠癌微转移。2、提示GC-C有希望用于结肠癌患者微转移的诊断指标,且优于CEA。

Expression of nitric oxide synthase and guanylate cyclase in the human ciliary body and trabecular meshwork

Background The role played by the nitric oxide （NO） signaling pathway in the aqueous humor dynamics is still unclear.This study was designed to investigate the expression and distribution of NO synthase （NOS） isoforms and guanylate cyclase （GC） in human ciliary body,trabecular meshwork and the Schlemm＇s canal.Methods Twelve eyes after corneal transplantation were used.Expression of three NOS isoforms （i.e.neuronal NOS （nNOS）,inducible NOS （iNOS） and endothelial NOS （eNOS）） and GC were assessed in 10 eyes by immunohistochemical staining using monoclonal or polyclonal antibody of NOS and GC.Ciliary bodies were dissected free and the total proteins were extracted.Western blotting was performed to confirm the protein expression of 3 NOS isoforms and GC.Results Expression of 3 NOS isoforms and GC were observed in the ciliary epithelium,ciliary muscle,trabecular meshwork and the endothelium of the Schlemm＇s canal.Immunoreactivity of nNOS was detected mainly along the apical cytoplasmic junction of the non-pigmented epithelium （NPE） and pigmented epithelial （PE） cells.Protein expressions of 3 NOS isoforms and GC were confirmed in isolated human ciliary body by Western blotting.Conclusions The expression of NOS isoforms and GC in human ciliary body suggest the possible involvement of NO and cyclic guanosine monophosphate （cyclic GMP,cGMP） signaling pathway in the ciliary body,and may play a role in both processes of aqueous humor formation and drainage.

The roles of cysteines in the heme domain of human soluble guanylate cyclase

Soluble guanylate cyclase（sGC） is a critical heme-containing enzyme involved in NO signaling.The dimerization of sGC subunits is necessary for its bioactivity and its mechanism is a striking and an indistinct issue.The roles of heme domain cysteines of the sGC on the dimerization and heme binding were investigated herein.The site-directed mutations of three conserved cysteines（C78A,C122A and C174S） were studied systematically and the three mutants were characterized by gel filtration analysis,UV-vis spectroscopy and heme transfer examination.Cys78 was involved in heme binding but not referred to the dimerization,while Cys174 was demonstrated to be involved in the homodimerization.These results provide new insights into the cysteine-related dimerization regulation of sGC.

Changes of Adenylate Cyclase and Guanylate Cyclase in the Frontal Cortex,Lenticula,Corpus Amygdaloideum,and Hippocampus in Morphine‑dependent Rats

To detect the changes of adenylate cyclase(AC)and guanylate cyclase(GC)in the four cerebral regions that are concerned with psychogenic dependence of morphine in rats,including the frontal cortex,lenticula,corpus amygdaloideum,and hippocampus.To discuss the relation between the expressions of AC and GC with the psychogenic dependence on morphine.Different periods of morphine‑dependent rat models were established,and enzyme histochemistry was used to detect the variations of AC and GC in four cerebral regions.Compared with the control group,AC and GC in all the morphine‑dependent groups increased.The data indicated that the amounts of AC and GC were significantly different between the morphine‑dependent groups and the control group when tested at periods of 1 week,2 weeks,4 weeks,and 8 weeks(P<0.05 or P<0.01).There were significant differences when comparing the 1‑week group with the 2‑week,4‑week,and 8‑week groups(P<0.05 or P<0.01).There were significant differences when comparing the 2‑week dependent group with the 4‑week dependent group or the 8‑week dependent group(P<0.05 or P<0.01).The activities of AC and GC increased in four cerebral regions of morphine‑dependent rats.The psychogenic dependence on morphine appears to be closely linked to the upgrade of AC and GC.

腹泻仔猪肠道菌群结构特征及肠道炎症因子、腺苷酸环化酶和鸟苷酸环化酶mRNA表达变化研究

选取同批次的21日龄仔猪,在断奶3 d后采集55份健康仔猪和37份腹泻仔猪的粪便样本,测定短链脂肪酸含量,采用高通量测序技术基于16S rRNA基因分析菌群结构,并分别选择6头腹泻和健康仔猪屠宰采集结肠黏膜样品对炎症因子、腺苷酸环化酶和鸟苷酸环化酶的mRNA表达水平进行检测。结果显示,与健康仔猪相比,腹泻仔猪粪便菌群的香农指数、Chao1指数显著(P<0.05)降低;在门水平上,变形菌门(Proteobacteria)和厚壁菌门(Firmicutes)的相对丰度显著提高,拟杆菌门(Bacteroidota)的相对丰度显著降低;在属水平上,大肠埃希菌-志贺菌属(Escherichia-Shigella)、乳酸杆菌属(Lactobacillus)和拟普雷沃氏菌属(Alloprevotella)的相对丰度显著升高,瘤胃球菌属(Ruminococcus)、瘤胃球菌科_uncultured(Ruminococcaceae_uncultured)、普雷沃氏菌科_NK3B31(Prevotellaceae_NK3B31_group)、理研菌科RC9属(Rikenellaceae_RC9_gut_group)、UCG-010_norank和狭义梭菌属_1(Clostridium_sensu_stricto_1)的相对丰度显著降低。菌群功能预测结果显示,与健康仔猪相比,腹泻仔猪中粪便菌群的糖酵解/糖异生、D-谷氨酰胺和D-谷氨酸代谢、D-精氨酸代谢通路的相对丰度显著升高,细菌趋化性,以及缬氨酸、亮氨酸和异亮氨酸的生物合成(valine, leucine and isoleucine biosynthesis)通路的相对丰度显著降低。腹泻仔猪粪便中的乙酸、丙酸和丁酸含量较健康仔猪显著降低,且乙酸含量与理研菌科RC9属、UCG-010_norank和瘤胃球菌科_uncultured的相对丰度呈显著正相关,丁酸含量与罗氏菌属(Roseburia)、不动杆菌属(Agathobacter)和狭义梭菌属_1的相对丰度呈显著正相关。与健康仔猪相比,腹泻仔猪肠道中促炎因子——肿瘤坏死因子-α(TNF-α)和白细胞介素-8(IL-8)的mRNA表达水平显著升高,抗炎因子——白细胞介素-10(IL-10)的mRNA表达水平显著降低(P<0.05),腺苷酸环化酶mRNA的表达水平显著升高。由此可见,断奶健康仔猪与腹泻仔猪的肠道菌群结构与功能存在显著差异,断奶后仔猪肠道中致病菌增加、有益菌减少和短链脂肪酸含量降低,以及促炎因子和腺苷酸环化酶mRNA水平的升高,导致仔猪发生腹泻。

维利西呱在心力衰竭中应用进展

心力衰竭的发生、发展涉及血管内皮功能障碍、炎症和氧化应激,这一病理生理过程会影响一氧化氮(nitric oxide,NO)-可溶性鸟苷酸环化酶(soluble guanylate cyclase,sGC)-环磷酸鸟苷-(cyclic guanosine monophosphate,cGMP)信号通路活性。维利西呱可通过刺激sGC提高cGMP水平,cGMP作为第二信使激活蛋白激酶、磷酸二酯酶和下游的信号通路,不仅舒张血管,改善冠状动脉血流量,而且可抑制炎症、心肌纤维化的进展,从而改善心衰患者的预后。目前维利西呱在射血分数降低的心力衰竭(heart failure with reduced ejection fraction,HFrEF)和射血分数保留的心力衰竭(heart failure with preserved ejection fraction,HFpEF)中均进行数个临床研究,其治疗心衰患者的安全性已被广泛证实,但有效性在不同类型的心衰患者有所差别。本文对心衰发生中的NO-sGC-cGMP通路的改变、维利西呱的作用机制及在心衰中的治疗进展进行综述。

慢性心力衰竭临床治疗的回顾及展望

慢性心力衰竭通常标志着大部分心血管疾病进入其终末阶段,具有患病率高、预后极其不利等特点。在药物治疗上,“金三角”方案被普遍视为治疗慢性心力衰竭的经典策略,近年来,随着大量的临床研究数据的公布,慢性心衰“新四联”疗法及可溶性鸟苷酸环化酶激动剂维立西呱等新型治疗药物开始应用于临床。一系列的生物标志物被发现,它们与慢性心衰患者的预后密切相关,如SERCA2a、中性粒细胞明胶酶相关脂质运载蛋白、生长分化因子15等。这些新疗法及生物标志物的发现有助于提高慢性心力衰竭患者的临床疗效及更好地预测其预后。本文就慢性心力衰竭临床治疗及生物标志物的研究及展望作一综述。