Expression Imbalance of Cholinergic M₂and M₃Receptors Contributes to the Motility Reduction of the Small Intestine in Spleen Qi Deficiency

Objective: To study roles of cholinergic M2 and M3 receptors in the motility reduction of small intestine (SI) in spleen qi deficiency. Methods: 16 male SD rats were randomly divided in the control group and spleen qi deficiency group (model group)—8 rats each group;spleen qi deficiency model of the improper diet and overfatigue was established;the SI propelling rate (SIPR) was used to evaluate the SI motility;ELISA was used to measure concentrations of acetylcholine (ACh), cyclic adenosine monophosphate (cAMP) and protein kinase A (PKA) in the SI tissue;immohistochemistry was employed to detect expressions of cholinergic M2 and M3 receptors. Results: Compared with those in the control group, SIPR was reduced;expression of M2 receptors was increased;and expression of M3 receptors and concentrations of cAMP and PKA were decreased, significantly, in the model group. Conclusions: Expression imbalance of cholinergic M2 and M3 receptors might contribute to the motility reduction of the SI in spleen qi deficiency.

Effect of organophosphorus insecticides on phosphorylation of the M_2 muscarinic acetylcholine receptor

BACKGROUND： Organophosphorus insecticides may promote the accumulation of acetylcholine at synapses and the neuromuscular junction by inhibiting acetylcholinesterase activity to cause disturbance of neural signal conduction and induce a toxic reaction. Organophosphorus insecticides may act on M2 muscarinic acetylcholine receptors, whose combination with G proteins is regulated by phosphorylation of G protein-coupled receptor kinase 2. OBJECTIVE： To investigate the effects of organophosphorus insecticides on the phosphorylation of G protein-coupled receptor kinase 2-mediated M2 muscarinic acetylcholine receptors and to reveal other possible actions of organophosphorus insecticides. DESIGN, TIME AND SETTING： An observational study, which was performed in the Central Laboratory of Shenyang Medical College, and Department of Physiological Sciences, College of Veterinary Medicine, Oklahoma State University from June 2002 to December 2004. MATERIALS： Paraoxon, parathion, chlorpyrifos, and chlorpyrifos oxon were provided by Chem Service Company, USA, [γ -p^32] ATP and [^35S]GTP γ S by New England Nuclear Life Science Products, and recombinant β 2-adrenergic receptor membrane protein by Sigma Company, USA. METHODS： The M2 muscarinic acetylcholine receptor was extracted and purified from pig brain using affinity chromatography. Subsequently, the purified M2 muscarinic acetylcholine receptor, G protein-coupled receptor kinase 2, and [γ -p^32] ATP were incubated with different concentrations of paraoxon and chlorpyrifos oxon together. The mixture then underwent polyacrylamide gel electrophoresis, and the gel film was dried and radioactively autographed to detect phosphorylation of the M2 muscarinic acetylcholine receptor. Finally, the radio-labeled phosphorylated M2 receptor protein band was excised for counting with an isotope liquid scintillation counter. MAIN OUTCOME MEASURES： Effects of chlorpyrifos oxon, paraoxon, chlorpyrifos, and parathion in different concentrations on the phosphorylation of the M2 muscarinic acetylcholine receptor; effects of chlorpyrifos oxon on the phosphorylation of the β -adrenergic receptor. RESULTS： Chlorpyrifos oxon could completely inhibit the phosphorylation of the M2 muscarinic acetylcholine receptor, and its IC50 was 70 μ mol/L. Chlorpyrifos could also inhibit the phosphorylation of the M2 muscarinic acetylcholine receptor. However, paraoxon and parathion could not inhibit the phosphorylation of the M2 muscarinic acetylcholine receptor. Chlorpyrifos oxon in different concentrations could also not inhibit the phosphorylation of the β 2-adrenergic receptor catalyzed by G protein-coupled receptor kinase 2. CONCLUSION： Different kinds of organophosphorus insecticides have different effects on the phosphorylation of the G protein-coupled receptor kinase 2-mediated M2 muscarinic acetylcholine receptor. Organophosphorus insecticides possibly have different toxic effects.

Expression and Significance of ECP, 25-(OH)D3 and M2 receptors in Children with Acute Attack of Asthma

Objective:To study the expression and significance of ECP, 25-(OH)D3 and M2 receptors in children with acute attack of asthma.Methods: Seventy children with bronchial asthma who first visited our hospital from September 2016 to September 2018 were divided into chronic persistence group, remission group and acute attack group. Thirty healthy children who underwent physical examination in our hospital were selected and divided into control group. The levels of ECP, 25-(OH) D3 and M2 receptors were analyzed by ELISA, and Pearson correlation analysis was performed.Results: Compared with the control group, the levels of ECP and M2 receptors in chronic persistence group, remission group and acute attack group increased, while the levels of 25-(OH)D3 decreased, with statistical difference (P<0.05). The levels of ECP and M2 receptors in acute attack group were higher than those in chronic persistence group, and the levels of 25-(OH)D3 were lower than those in chronic persistence group (P<0.05). The levels of ECP and M2 receptors in acute attack group were higher than those in remission group, and the levels of 25-(OH)D3 were lower than those in remission group (P<0.05). Compared with mild children, the levels of ECP and M2 receptors increased and 25-(OH)D3 decreased in moderate and severe children (P<0.05). Compared with moderate children, the levels of ECP and M2 receptors increased and 25-(OH)D3 decreased in severe children (P<0.05).There was a negative correlation between ECP and 25-(OH)D3 (r=-0.380, P=0.038);a negative correlation between 25-(OH)D3 and M2 receptor (r=-0.448,P=0.013);and a positive correlation between ECP and M2 receptor (r=0.450,P=0.013).Conclusions:The expression of ECP and M2 receptors increased during the acute attack of bronchial asthma in children, while the expression of 25-hydroxyvitamin D3 decreased during the acute attack of bronchial asthma in children. The correlation among ECP, 25-(OH) D3 and M2 receptors is significant in the clinical diagnosis of acute attack of bronchial asthma in children.

Research on Autoantibodies Against Myocardialβ_1-adrenergic and M_2 Cholinergic Receptors in Patients With Chronic Keshan Disease

Objectives To explore the relationship between serum autoantibodies against myocardial β1-adrenergic, M2-cholinergic receptors and chronic Keshan disease （CKD）. Methods The second extracellular loops of β1 and M2 receptors on human cardiomyocytes were used as the antigens. Enzyme linked immunosorbent assay （ELISA） was applied to determine serum autoantibodies against myocardial β1 and ME receptors in 32 CKD patients. 31 healthy subjects from endemic area were selected as the control. Results Positive rate of autoantibodies against myocardial β1 adrenergic （51.3%, 17/32） and M2 cholinergic （56.3% , 18/32） receptors were significantly higher than those in the control （9.7%, 3/ 31; 12.9%, 4/31） （both P〈 0.01）. Both positive rate and titers of above autoantibodies in NYHA Ⅱ - Ⅲ CKD patients were significantly higher than those in NYHA Ⅳ, demonstrating an apparently positive correlation between serum antibodies against myocardial β1 and M2 receptors （r=0.95）. Conclusions Autoantibodies against myocardial β1 and M2 receptors were found in sera of CKD patients; distribution of positive rate and titers of the autoantibodies in CKD patients in various NYHA are significantly different. classes of cardiac function

老年扩张型心肌病与心脏β_1和M_2受体自身抗体的研究

目的 探讨心脏β1和M2 受体的自身抗体在老年扩张型心肌病发生、发展中的临床意义。方法 以细胞外第二环表位肽段的合成肽作为抗原 ,应用酶联免疫吸附测定 (ELISA)技术 ,检测 32例老年扩张型心肌病 (seniledilatedcardiomyopathy,SDCM)、2 6例非老年扩张型心肌病 (non senileDCM ,NSDCM)和 2 0名正常对照的老年人。结果 SDCM组心脏 β1受体自身抗体的阳性率为 2 8.1% (9/32 ) ,NSDCM组为 5 3 .8% (14/2 6 ) ,对照组为 15 .0 % (3/2 0 ,P <0 .0 5 ) ;SDCM组心脏M2 受体自身抗体的阳性率为 31.3% (10 /32 ) ,NSDCM组为 5 7.7% (15 /2 6 ) ,对照组为 2 0 .0 % (4/2 0 ,P<0 .0 1) ;SDCM组心功能Ⅱ～Ⅲ级的两种抗体阳性率及抗体滴度与心功能Ⅳ级比较无明显差异。NSDCM组心功能Ⅱ～Ⅲ级的阳性率及抗体滴度明显高于心功能Ⅳ级。结论 心脏 β1与M2 受体自身抗体的产生与SDCM相关 ,但相关程度低于NSDCM组 ;提示在SDCM患者心功能状态多属晚期的病程中 ,心脏 β1和M2 受体自身抗体的产生 。

胆碱能M_2受体激动剂及拮抗剂对大鼠脚桥核神经元电活动的影响

目的 在体水平上观察选择性胆碱能M2 受体激动剂oxotremorine和拮抗剂methoctramine对大鼠PPN神经元自发放电频率的影响。方法 采用玻璃微电极细胞外记录和脚桥核 (pedunculopontinenucleus ,PPN)内微量注射法。 结果 11个神经元在PPN内微量注射高浓度 (每 2 0 0nl含 4 μg)oxotremorine后 ,10个神经元被兴奋 ,放电频率较注射前升高 (2 82± 5 9) % ,1个神经元放电频率无明显变化 ;低浓度 (每 2 0 0nl含 0 .2 μg)oxotremorine注射后 ,11个神经元中 ,有 6个神经元被抑制 ,放电频率较注射前降低 (98± 2 ) % ,5个神经元被兴奋 ,放电频率较前对照升高(6 80± 32 4 ) %。 12个神经元在PPN内微量注射高浓度 (每 2 0 0nl含 4 μg)methoctramine后 ,4个神经元被兴奋 ,放电频率较前对照升高 (4 0 9± 133) % ,6个神经元被抑制 ,放电频率较注射前降低 (86± 8) % ,2个放电频率无显著变化 ;低浓度 (每 2 0 0nl含 0 .4 μg)methoctramine注射后 ,12个神经元中 ,有 5个神经元被兴奋 ,放电频率较前对照升高 (117± 15 ) % ,6个神经元被抑制 ,放电频率较注射前降低 (79± 11) % ,1个放电频率未受明显影响。 结论 胆碱能M2

^(99)Tc^(m)标记多巴胺D_(2)受体配体的合成,标记及生物分布研究

首次合成了 3种苯酰胺类D2 受体配体 :N [(2 巯基 )乙基 ] 2 ,3 二甲氧基苯甲酰胺 (MEDM BZM) ,N [(2 巯基 )乙基 ] 5 溴 2 ,3 二甲氧基苯甲酰胺 (MEBDM BZM ) ,N [(2 巯基 )乙基 ] 3 乙氧基苯甲酰胺 (MEE BZM) ,光谱数据与结构相符。用配体交换法与 3 硫杂 1,5 戊二硫醇共同配位合成了中性脂溶性的“3+ 1”型混配99Tcm 螯合物 ,标记率大于 85 %。

用转染m2胆碱受体基因的CHO细胞观察知母皂甙元的作用

目的观察知母甾体皂甙元 (sarsasapogenin ,SAR)对M2 受体亚型的调节作用。 方法采用转染了m2胆碱受体基因的CHO细胞为模型 ,以非选择性的3H -QNB作单点放射配基结合分析。 结果CHOm2细胞受体密度在培养 48h达顶峰 ,以后呈进行性下降。SAR对下降的CHOm2细胞M2 受体密度有明显的上调作用 ,这一作用有一定浓度依赖性。 结论SAR对下降的M2 受体密度具有上调作用。

人粪便中OSMR和TFPI2基因甲基化在结直肠癌诊断中的意义

目的:探讨检测人粪便中抑瘤素M型受体(OSMR)基因和组织因子途径抑制子2(TFPI2)基因甲基化对于结直肠癌及腺瘤诊断的可行性及临床意义.方法:从60例结直肠癌患者和17例腺瘤患者及30名正常对照者的粪便中分别提取DNA,应用甲基化特异性PCR方法检测人粪便中OSMR和TFPI2基因的甲基化状态.结果:结直肠癌患者粪便中OSMR及TFPI2基因甲基化检出率分别高于腺瘤患者和正常对照者[OSMR:35%(21/60)vs12%(2/17),7%(2/30);TFPI2:70%(42/60)vs18%(3/17),3%(1/30);均P<0.01].二者联合检测甲基化检出率为81.7%(49/60),特异性90%.结论:检测粪便中OSMR和TFPI2基因甲基化在结直肠癌诊断和筛查中有潜在的应用价值.

心肌M_2胆碱受体抗体对大鼠心房及心室肌cAMP含量的影响

目的 :了解心肌M2 胆碱受体抗体 (M2 Ab)对大鼠心房和心室肌cAMP含量的影响 ,并与M2 胆碱受体激动剂卡巴可 (Carb)的作用进行了对比观察。方法 :采用离体生化放射免疫分析法测定M2 Ab及M2 胆碱受体激动剂Carb对心肌cAMP含量的影响。结果 :①M2 Ab及Carb两者均可剂量依赖性抑制异丙肾上腺素 (Isoproterenol,Iso)所刺激的大鼠心房及心室肌cAMP的增加。卡巴可浓度为 2 μmol/L ,10 μmol/L ,5 0 μmol/L时可分别抑制Iso所刺激的cAMP含量 (8.5± 1.2 ) % ,(16 .2± 1.4) % ,(2 9.5± 2 .1) % ,而M2 Ab浓度为 5 0nmol/L ,10 0nmol/L ,40 0nmol/L时 ,可分别抑制 (6 .1± 0 .6 ) % ,(17.3± 1.8) % ,(31.7± 3.1) % (P <0 .0 1)。②Carb(10 μmol/L)及M2 Ab(10 0nmol/L)两者可分别抑制基础cAMP(49.2± 4.3) %和 (6 4.3± 5 .1) %。③M受体阻断剂阿托品 (Atr) (1.5 μmol/L)不但可阻断Carb对Iso的抑制反应 ,亦能阻断M2 Ab的这种反应。而相应的抗原性肽段也能阻断M2 Ab的这种反应。结论 :M2 Ab抑制Iso引起的心室肌细胞cAMP生成量的增加反应 ,类似于M受体激动剂Carb ,两者效应均通过作用于M2 受体途径实现。

新蛋白质合成介导知母活性成分对M_2受体稳定性的调节作用

目的探讨知母活性成分ZMS提高CHOm2细胞毒蕈碱样乙酰胆碱2型受体(M2受体)mRNA表达的机制。方法体外培养至80%～90%融合的CHOm2细胞分为ZMS1组(单纯添加1×10-5mol/LZMS作用24h)、ZMS2组(添加1×10-5mol/LZMS作用24h后加入1μg/mL环己酰亚胺作用12h)、ZMS3组(加入1μg/mL环己酰亚胺预处理4h后加入1×10-5mol/LZMS作用24h),以上各组分别设立对照组(以等体积DMSO替代ZMS,其他处理与相应ZMS组相同)。各组细胞培养基中均加入放线菌素D抑制mRNA合成,于不同时间点收集CHOm2细胞,Real-time PCR检测M2受体mRNA相对表达量并计算半衰期。结果与相应对照组比较,ZMS1组和ZMS2组CHOm2细胞M2受体mRNA的半衰期明显延长,分别为(4.75±0.54)hvs(2.13±0.23)h和(5.43±1.13)hvs(2.46±0.09)h(均P<0.05);添加1μg/mL环己酰亚胺预处理的ZMS3组CHOm2细胞M2受体mRNA半衰期的(3.06±0.23)h与其相应对照组的(3.00±0.20)h比较,差异无统计学意义(P>0.05)。结论ZMS提高M2受体mRNA的稳定性需要有新蛋白质合成的参与。

α-、β-雌二醇和中药有效成分ZDY101对CHOm_2转基因细胞M_2受体的影响

本文用细胞培养技术 ,对比观察了α -雌二醇 (α -E2 )、β -雌二醇 (β -E2 )和滋阴药有效成分ZDY10 1对转染M2 受体基因的CHO细胞M2 受体密度的影响。在CHOm2 转基因细胞培养 2 4h后 ,加入不同浓度的α -E2 、β -E2 或ZDY10 1。继续培养 4 8h后收集细胞 ,用3 H -QNB单点法测定M2 受体密度。发现α-E2 及 β -E2 在浓度为 1× 10 -5mol/L时 ,M2 受体密度明显高于对照组 ,与相同浓度的ZDY10 1作用相仿。以上结果提示 :由于α -E2 及β-E2 对M2 受体密度的作用相似 ,所以E2 对M2 受体的调整作用 ,其受体后的信息传递机制很可能与对雌性器官的调整作用是不同的 ;由于ZDY10 1与E2 结构上和调节M2 受体的作用有类似处 ,它和E2 及E2

糖尿病肾病患者血清TRPM7、Sirtuin-1与钙磷代谢、颈动脉钙化的相关性

目的探讨糖尿病肾病(DN)患者血清瞬时受体电位通道7(TRPM7)、沉默调节蛋白-1(Sirtuin-1)与钙磷代谢、颈动脉钙化的相关性。方法选取2020年12月—2022年11月成都大学附属医院收治的97例DN患者作为DN组,另取同期在该院就诊的120例2型糖尿病患者作为对照组。采用实时荧光定量聚合酶链反应检测血清TRPM7的表达,酶联免疫吸附试验检测血清Sirtuin-1水平。采用Pearson法分析DN患者血清TRPM7、Sirtuin-1水平与钙磷代谢的相关性,并通过多因素Logistic逐步回归模型分析DN患者颈动脉钙化的危险因素。结果DN组血肌酐、尿素氮、血清TRPM7、血磷、颈动脉钙化率高于对照组(P<0.05)。DN组Sirtuin-1、血钙低于对照组(P<0.05)。Pearson相关性分析结果显示,DN患者血清TRPM7与血钙呈负相关(r=-0.247,P=0.000),与血磷呈正相关(r=0.415,P=0.000);DN患者血清Sirtuin-1与血钙呈正相关(r=0.367,P=0.000),与血磷呈负相关(r=-0.505,P=0.000)。钙化组DN患者糖尿病病程、空腹血糖、血肌酐、血磷、TRPM7水平高于非钙化组(P<0.05),血镁、血钙、Sirtuin-1水平低于非钙化组(P<0.05)。多因素Logistic逐步回归分析结果显示:血镁≤0.89mmol/L[OR=2.277(95%CI:1.521,3.410)]、TRPM7≥1.41[OR=3.019(95%CI:1.901,4.795)]、Sirtuin-1≤8.81 ng/mL[OR=2.591(95%CI:1.657,4.051)]是DN患者颈动脉钙化的危险因素(P<0.05)。结论DN患者血清TRPM7升高、血清Sirtuin-1降低,两者与钙磷代谢密切相关,且血清TRPM7高表达、Sirtuin-1低表达是DN患者颈动脉钙化的危险因素。

特发性膜性肾病与M型磷脂酶A2受体

膜性肾病是导致成人患者原发性肾病综合征的常见原因.其中特发性膜性肾病约为80%.膜性肾病的发病系循环中的自身抗体识别肾小球足细胞的靶抗原,抗原抗体结合后,在上皮下形成免疫复合物,激活补体形成膜攻击复合物,导致基底膜和肾小球滤过屏障受损,出现蛋白尿[1,2].近半个世纪以来,人们针对特发性膜性肾病的靶抗原作了大量研究,并取得了实质性进展,其中,M型磷脂酶A2受体（M-type phospholipase A2 receptor,PLA2R）是近年来研究的热点,现就PLA2R与特发性膜性肾病之间的关系综述如下.

瞬时受体电位阳离子通道亚家族M成员2在小鼠肝缺血再灌注损伤模型中的作用及机制

目的:观察瞬时受体电位阳离子通道亚家族M成员2(transient receptor potential cation channel subfamily M member 2,TRPM2)在小鼠肝缺血再灌注损伤(hepatic ischemia-reperfusion injury,HIRI)模型中的作用及可能的机制。方法:60只成年雄性C57BL/6小鼠随机分为假手术组(S组)、模型组(M组)、TRPM2腺病毒干扰载体预处理组(T组)和TRPM2腺病毒对照载体预处理组(C组)(均n=15)。取各组小鼠灌注前肝组织,采用荧光显微镜观察腺病毒感染效率,利用real-time PCR检测腺病毒对TRPM2的沉默效率。各组小鼠分别于再灌注2,4和8 h抽取腹主动脉血并获取肝组织,分别检测血清中谷丙转氨酶(alanine amino-transferase,ALT)和谷草转氨酶(aspartate amino-transferase,AST)活性。采用HE染色观察肝组织病理学变化;蛋白质印迹法检测肝中TRPM2和Rac家族小GTP酶1(Rac family small GTPase 1,RAC1)蛋白质的表达量变化;并通过酶联免疫吸附试验检测肝中丙二醛(malondialdehyde,MDA)、超氧化物歧化酶(superoxide dismutase,SOD)及髓过氧化物酶(myeloperoxidase,MPO)活性的变化。结果:与S组和M组相比,T组和C组小鼠肝组织可见大量绿色荧光。与S组、M组及C组相比,T组小鼠肝组织中TRPM2 mRNA的表达量显著降低(均P<0.05)。光镜下S组小鼠肝细胞形态正常;M组和C组小鼠肝窦扩张和淤血、肝细胞变性、小叶中央坏死及大量炎症细胞浸润;与M组和C组相比较,T组小鼠肝细胞受损程度明显减轻。与S组相比较,M组、T组及C组小鼠血清中ALT及AST活性在再灌注2,4和8 h均显著升高(均P<0.05);与M组和C组相比较,T组小鼠血清中ALT及AST活性在再灌注2,4和8 h均显著降低(均P<0.05)。与M组和C组相比较,T组小鼠中SOD活性在再灌注2,4和8 h均显著升高(均P<0.05),而MDA和MPO活性均显著降低(均P<0.05)。T组小鼠肝组织中TRPM2和RAC1蛋白质表达量在再灌注2,4和8 h较M组和C组均显著降低(均P<0.05)。结论:TRPM2腺病毒干扰载体预处理能有效沉默小鼠肝组织中TRPM2基因表达,并能减轻HIRI,该机制可能与抑制氧化应激和降低RAC1蛋白质表达水平有关。

血清M2-AAb、β1-ARAb水平与肥厚型心肌病患者左心功能的相关性研究

目的探讨肥厚型心肌病患者血清中M2乙酰胆碱能受体自身抗体(M2-AAb)、β1肾上腺素能受体自身抗体(β1-ARAb)水平与肥厚型心肌病患者左心功能的相关性。方法选取2017年1月至2019年3月于该院心血管内科住院接受治疗的126例肥厚型心肌病患者为肥厚型心肌病组,选取同期的107例体检健康者作为对照组。采用ELISA法检测肥厚型心肌病患者血清中M2-AAb、β1-ARAb水平;采用多普勒心脏超声检测左心功能各指标水平;分析肥厚型心肌病患者血清中M2-AAb、β1-ARAb水平的相关性;分析肥厚型心肌病患者血清中M2-AAb、β1-ARAb水平与左心功能指标的相关性。结果肥厚型心肌病组血清中M2-AAb、β1-ARAb水平明显高于对照组(P<0.05);两组左心室射血分数(LVEF)比较,差异无统计学意义(P>0.05)。肥厚型心肌病组左室舒张末期内径(LVD)、二尖瓣舒张早期血流速度峰值(E)/二尖瓣瓣环组织多普勒速度(E′)、左室舒张末期左心房容积(LAV)、左房容积指数(LAVI)明显高于对照组(P<0.05),E/二尖瓣舒张晚期血流速度峰值(A)低于对照组(P<0.05)。肥厚型心肌病患者血清中M2-AAb、β1-ARAb水平呈正相关;肥厚型心肌病患者血清中M2-AAb、β1-ARAb水平与LVD、E/E′、LAV、LAVI均呈正相关(P<0.05),与E/A呈负相关(P<0.05)。结论血清M2-AAb、β1-ARAb水平与肥厚型心肌病患者左心功能指标具有一定相关性。血清M2-AAb、β1-ARAb水平联合左心功能检测在肥厚型心肌病的早期诊断及病程评估中具有较高的应用价值。

高血压性心脏病抗G-蛋白偶联β_1-肾上腺素能受体与M_2-胆碱能受体自身抗体的初步研究

目的抗心肌β１和Ｍ２的自身抗体是否与高血压性心脏病有关。方法以心脏Ｇ－蛋白偶联受体β１和Ｍ２细胞外第二环表位肽段的合成肽作为抗原，应用酶联免疫吸附测定（ＥＬＩＳＡ）技术检测４４例高血压性心脏病（ＨＣＤ）患者、３６例单纯性高血压患者和４１例正常人（对照组）血清中抗β１和Ｍ２受体的自身抗体。结果抗心肌β１受体自身抗体的检出率，高血压性心脏病患者为４７．７％（２２／４４），显著高于高血压患者１１．１％（４／３６）与正常人１２．１（５／４１）；抗心肌Ｍ２受体自身抗体的检出率，高血压性心脏病患者为４５．５％（２０／４４），显著高于高血压患者８．３％（３／３６）与正常人９．８％（４／３６）。高血压性心脏病患者血清中抗β１和Ｍ２受体的自身抗体滴度分别为１∶９６与１∶１０３，远高于单纯性高血压和对照组的１∶４０与１∶２４的相应抗体滴度（Ｐ＜０．０５）。结论高血压性心脏病患者不仅存在抗心肌β１和Ｍ２受体的自身抗体而且其抗体滴度也明显高于单纯性高血压及正常人，检测该抗体对预测原发性高血压患者是否并发心肌病变，可能有一定的参考价值。

^(99)Tc^(m)-3PRGD_(2)单光子发射计算机断层显像在大鼠乳腺癌骨移植瘤放疗疗效评价中的价值观察

目的观察^(99)Tc^(m)-3PRGD_(2)单光子发射计算机断层(SPECT)显像在大鼠乳腺癌骨移植瘤放疗疗效评价中的价值。方法50只Wistar大鼠通过骨髓腔内注入含有大鼠乳腺癌细胞的腹水混悬液建立胫骨移植瘤模型,最终成瘤30只。将30只乳腺癌骨移植瘤大鼠按随机数字表法分为对照组、低剂量放疗组、高剂量放疗组各10只,分别于骨移植瘤部位行0 Gy、5 Gy、25 Gy的单次大剂量直线加速器放疗,各组分别于放疗前及放疗结束后第10天尾静脉注射^(99)Tc^(m)-3PRGD_(2),1 h后行SPECT显像并计算骨移植瘤部位放射性计数与对侧相应部位同等大小区域的放射性计数比值(T/NT)。显像结束后处死大鼠,采用HE染色观察大鼠胫骨组织病理改变,采用免疫组织化学法观察骨移植瘤组织整合素αⅤβ_(3)受体表达情况。采用Spearman相关性分析T/NT与整合素αⅤβ_(3)受体阳性细胞表达的关系。结果各组放疗前行^(99)Tc^(m)-3PRGD_(2)SPECT显像,骨移植瘤部位均可见显像剂浓聚影,浓聚程度无明显差异;各组放疗前T/NT比较无统计学差异。各组放疗后行^(99)Tc^(m)-3PRGD_(2)SPECT显像,显像剂浓聚程度对照组>低剂量放疗组>高剂量放疗组;各组放疗后T/NT对照组>低剂量放疗组>高剂量放疗组(P均<0.05)。HE染色可见各组胫骨组织均有骨结构破坏,对照组内肿瘤细胞密度高于高、低剂量放疗组,高、低剂量放疗组内有大量肿瘤细胞坏死,其中以高剂量放疗组肿瘤细胞坏死最多。对照组、低剂量放疗组、高剂量放疗组骨移植瘤组织整合素αⅤβ_(3)受体阳性率对照组>低剂量放疗组>高剂量放疗组(P均<0.05)。Spearman相关性分析显示,T/NT与αⅤβ_(3)受体阳性细胞表达呈正相关(r=0.847,P<0.01)。结论^(99)Tc^(m)-3PRGD_(2)SPECT显像指标变化与骨移植瘤病理改变一致,用于大鼠乳腺癌骨移植瘤放疗疗效评价的效果良好。

对氧磷和氧毒死蜱对大鼠脑毒蕈碱乙酰胆碱M_2受体磷酸化的影响

目的研究有机磷类杀虫剂对氧磷(PO)和氧毒死蜱(CPO)对大鼠脑G蛋白偶联受体激酶2介导的毒蕈碱乙酰胆碱M2受体磷酸化的影响。方法制备亲和层析柱;利用亲和层析方法从大鼠脑中纯化毒蕈碱乙酰胆碱M2受体;将纯化的毒蕈碱乙酰胆碱M2受体或β2-肾上腺素受体、G蛋白偶联受体激酶-2、[γ-p32]ATP与对氧磷(PO)、氧毒死蜱(CPO)共同保温,聚丙烯酰胺凝胶电泳分离蛋白,放射性自显影检测M2受体磷酸化结果。结果氧毒死蜱完全抑制大鼠脑M2受体的磷酸化,其半数抑制浓度为(IC50)70μmol/L;对氧磷不抑制毒蕈碱乙酰胆碱M2受体的磷酸化;氧毒死蜱和对氧磷都不抑制β-肾上腺素受体的磷酸化。结论氧毒死蜱有选择性地抑制大鼠脑毒蕈碱乙酰胆碱M2受体的磷酸化,说明某些有机磷杀虫剂的毒性作用存在其他靶分子或作用途径。

TET2上调IRAK-M表达促进巨噬细胞内毒素耐受

目的:研究TET2蛋白(ten-eleven translocation 2)对巨噬细胞白介素-1受体相关激酶-M(interleukin-1 receptor-associated kinase-M,IRAK-M)表达的影响,探讨细菌内毒素(endotoxin/lipopolysaccharide,LPS)刺激诱导TET2表达的上游信号通路。方法:用LPS刺激小鼠巨噬细胞系RAW264.7诱导内毒素耐受,qPCR和Western blot检测LPS刺激不同时间点和内毒素耐受时IRAK-M和TET2表达;用siRNA干扰TET2表达,qPCR和Western blot检测对IRAK-M表达的影响;用促分裂原活化的蛋白激酶(mitogen-activated protein kinase,MAPK)信号通路抑制剂预处理细胞,再用LPS刺激,qPCR和Western blot检测对TET2表达的影响。结果:TET2蛋白和IRAK-M在LPS刺激RAW264.7细胞诱导内毒素耐受后仍持续表达,且表达模式都和细胞因子表达模式相反;干扰TET2表达抑制IRAK-M m RNA(P=0.000)和蛋白水平表达;抑制MAPK信号通路抑制TET2表达。结论:巨噬细胞炎症反应过程中MAPK信号通路上调TET2表达,TET2通过促进IRAK-M表达促进内毒素耐受。