半胱胺盐酸盐对仔猪胃黏膜细胞H^+-K^+-ATPase活性和生长抑素表达的影响

将分离的仔猪胃粘膜细胞分为4组,在含10%胎牛血清的DM EM高糖培养液中培养24 h后,分别在新鲜的基础培养液中添加0(对照组)、0.001(低水平组)、0.01(中水平组)和0.1(高水平组)g/L的半胱胺盐酸盐,继续培养20 h后收集细胞,测定细胞H+-K+-ATPase活性,同时用相对定量RT-PCR法测定细胞H+-K+-ATPase和生长抑素(SS)mRNA的相对丰度。结果表明:(1)低水平的半胱胺盐酸盐对H+-K+-ATPase的表达和活性没有影响(P>0.05),但中、高水平的半胱胺盐酸盐显著提高了H+-K+-ATPase的表达和活性(P<0.05),其中H+-K+-ATPase mRNA的相对丰度分别提高了36%和44%,H+-K+-ATPase活性分别提高了57%和53%。(2)低水平半胱胺盐酸盐对SS mRNA的表达没有影响(P>0.05),中、高水平的半胱胺盐酸盐显著提高了SS mRNA的相对丰度(P<0.05),提高幅度均为52%。以上结果提示半胱胺盐酸盐可增强体外培养的仔猪胃黏膜细胞H+-K+-ATPase的表达及活性,而这一作用可能由SS所介导。

肉碱对不同强度运动大鼠骨骼肌线粒体呼吸链H^+-K^+-ATPase活性的影响

目的:观察左旋肉碱对不同强度递增负荷跑台运动后大鼠骨骼肌线粒体H^+-K^+-ATPase活性的影响。方法:健康雄性Wistar大鼠40只,随机分为8组(n=5):对照组(A)、肉碱组(L)、运动组(E1、E2、E3)和运动结合肉碱组(LE1、LE2、LE3)。差速离心法提取骨骼肌线粒体,分光光度计测定骨骼肌线粒体H^+-K^+-ATPase活性。结果:与A组相比,L组大鼠H^+-K^+-ATPase活性升高31.18%;E1组提高44.46%(P<0.05);LE1组提高64.50%(P<0.01);E2、LE2组分别提高了63.65%、71.15%(P<0.01);E3组活性下降21.68%;LE3组提高57.81%(P<0.05)。与L组比较,LE1、LE2组提高了48.42%、58.08%(P<0.05);LE3组提高38.70%。与E1组相比,LE1组提高了36.07%;与E2相比,LE2组提高了20.65%;,与E3组相比,LE3组提高66.96%(P<0.01)。结论:肉碱干预后大鼠骨骼肌线粒体H^+-K^+-ATPase活性明显增强,大鼠运动能力明显提高。

Cysteamine increases expression and activity of H^1-K^+-ATPase of gastric mucosal cells in weaning piglets

AIM: To determine the in vivo andin vivo effects of cysteamine (CS) on expression and activity of H+-K+-ATPase of gastric mucosal cells in weaning piglets.METHODS: Eighteen litters of newborn Xinhuai piglets were employed in the in vivo experiment and allocated to control and treatment groups. From 12 d of age (D12), piglets in control group were fed basal diet, while the treatment group received basal diet supplemented with 120 mg/kg CS. Piglets were weaned on D35 in both groups. Six piglets from each group (n = 6) were slaughtered on D28 (one week before weaning), D35(weaning), D36.5, D38, D42, and D45 (36 h, 72 h,one week and 10 d after weaning), respectively. Semiquantitative RT-PCR was performed todetermine the levels of H+-K+-ATPase mRNA in gastric mucosa. H+-K+-ATPase activity in gastric mucosa homogenate was also determined. Gastric mucosal epithelial cells from piglets through primary cultures were used to further elucidate the effect of CS on expression and activity of H+-K+-ATPase in vivo. Cells were treated for 20 h with 0.001,0.01, and 0.1 mg/mL of CS (n = 4), respectively. The mRNA expression of H+-K+-ATPase and somatostatin (SS)as well as the H+-K+-ATPase activity were determined.RESULTS: in vivo, both mRNA expression and activity of H+-K+-ATPase in gastric mucosa of control group exhibited a trend to increase from D28 to D45, reaching a peak on D45, but did not show significant age differences. Furthermore, neither the mRNA expression nor the activity of H+-K+-ATPase was affected significantly by weaning. CS increased the mRNA expression of H+-K+-ATPase by 73%, 53%, 30% and 39% on D28(P = 0.014), D35 (P = 0.017), D42 (P = 0.013) and D45(P = 0.046), respectively. In accordance with the mRNA expression, H+-K+-ATPase activities were significantly higher in treatment group than in control group on D35(P = 0.043) and D45 (P = 0.040). In vivo, CS exhibited a dose-dependent effect on mRNA expression and activity of H+-K+-ATPase. Both H+-K+-ATPase mRNA expression and activity in gastric mucosal epithelial cells were significantly elevated after 20 h of exposure to the moderate (H+-K+-ATPase expression: P=0.03; H+-K+-ATPase activity: P = 0.014) and high concentrations (H+-K+-ATPase expression: P=0.017; H+-K+-ATPase activity:P = 0.022) of CS. Significant increases in SS mRNA expression were observed to accompany the elevation of H+-K+-ATPase expression and activity induced by the moderate (P = 0.024) and high concentrations (P = 0.022) of CS. Low concentration of CS exerted no effects either on expression and activity of H+-K+-ATPase or on SS mRNA expression in cultured gastric mucosal epithelial cells.CONCLUSION: No significant changes are observed in mRNA expression and activity of H+-K+-ATPase in gastric mucosa of piglets around weaning from D28 to D45. CS increases expression and activity of gastric H+-K+-ATPase in vivo and in vivo. SS is involved in mediating the effect of CS on gastric H+-K+-ATPase expression and activity in weaning piglets.

盐度对军曹鱼稚鱼血液生理生化及鳃Na^+-K^+ ATPase活性的影响

军曹鱼稚鱼[体重(6.52±0.71)g]在适应不同盐度(5、10、20、30和37)14 d后盐度5和10处理组特定生长率(SGR)显著低于其它组(P(0.05),且该两组血红蛋白、血细胞比容和红细胞数也显著低于盐度30和37组,而血清皮质醇和乳酸含量则明显高于盐度30和37组。此外,低盐度组中稚鱼血糖有升高趋势,门冬氨酸氨基转移酶(AST)含量随盐度降低而升高,但碱性磷酸酯酶(ALP)变化则相反。血清渗透压、Na+和C l-离子浓度与盐度呈正相关,而K+浓度呈负相关。鳃NKA活性在盐度20组中最低,在盐度10组中最高。研究显示军曹鱼稚鱼有较强的盐度适应能力,适度降低盐度并不影响其生长,但在过低盐度中仍呈应激反应,且盐度变化还可影响多项血液生理生化指标。

植物质膜H^+-ATPase的研究进展

质膜H+-ATPase参与植物细胞的物质跨膜转运、细胞的伸长生长、气孔的开闭以及植物对环境胁迫的响应等生理过程,是植物生命活动的“主宰酶”。其活性调节涉及激素、环境因子等多种因素,可发生在转录、翻译和酶分子等多级水平。因此,在植物生长发育过程中,质膜H+-ATPase活性的调节对生理活动起重要作用。本文就植物质膜H+-ATPase的结构特征、生理功能、活性变化及其调节机理等的研究进展进行综述,以进一步揭示该酶的生理功能及其调节机理与植物生命活动过程的关系。

盐胁迫对胡杨液泡膜H^+ATPase水解活性的影响

胡杨细胞经 50mmol·L- 1 NaCl处理 1 0d后 ,泡膜液H+ ATPase,PPiase水解活性都增加了 ,说明胡杨具有盐生植物的特性。盐胁迫对专一性抑制剂bafilomycinA1 ,DCCD更敏感 ,说明盐处理下胡杨液泡膜H+ ATPase与bafilomycinA1 ,DCCD结合位点上的构象可能发生了一定的变化。从Mg2 + ,ATP依赖性 ,NO3- 和bafilomycinA1 抑制特性、Cl- 激活特性证明胡杨液泡膜H+ ATPase是典型的V H+ ATPase。盐胁迫后 ,对底物ATP的亲和力增强。

外源一氧化氮供体对感染轮纹病菌后梨质膜H^+—ATPase及抗氧化酶活性的影响

梨叶片感染轮纹病菌5d后,用不同浓度的一氧化氮供体硝普钠(SNP)处理,测定了质膜H+—ATPase及抗氧化酶活性的变化。结果表明:浓度为0.3mmol/L SNP处理可提高H+—ATPase、抗坏血酸过氧化物酶(APX)、愈创木酚过氧化物酶(GPX)和谷胱甘肽还原酶(GR)活性,降低脂氧合酶(LOX)活性;浓度为0.1mmol/L和0.6mmol/L SNP处理则对其影响效果不明显;在同一浓度SNP处理组中,随处理时间的延长,其变化不同,较低浓度的SNP可缓解轮纹病菌对梨的伤害作用。

半胱胺对断奶前后仔猪胃粘膜H^-+K^+-ATPase表达和活性的影响

实验选取新生仔猪18窝, 随机分为实验组和对照组各9窝, 自12日龄起, 对照组饲喂基础乳猪料, 实验组在基础饲料中添加半胱胺120 mg/kg饲料, 仔猪均于35日龄断奶。分别于断奶前1 周、断奶当天、断奶后36 h、72 h、1周以及断奶后10 d屠宰仔猪取样, 每个时间点随机选取对照组和试验组各6头仔猪, 用相对定量RT PCR方法测定不同日龄仔猪胃组织中H+ K+ ATPase mRNA 表达的相对含量, 并同时测定H+ K+ ATPase的活性。结果表明: (1) 对照组仔猪在断奶前1 周至断奶后10 d, H+ K+ ATPase mRNA相对含量和H+ K+ ATPase活性有上升趋势, 两组仔猪在断奶后10 d H+ K+ ATPase mRNA相对含量和活性均达到最高水平, 但总体不表现显著的年龄差异; (2) 半胱胺能明显提高仔猪胃粘膜中H+ K+ ATPase mRNA的表达, 在断奶前1 周、断奶当天、断奶后1周和断奶后10 d均出现显著差异。半胱胺也能明显提高H+ K+ ATPase 的活性, 在断奶当天和断奶后10 d, H+ K+ ATPase 的活性分别被提高32 3%和18 3%; (3) 观察期内对照组和实验组H+ K+ ATPase mRNA水平和H+ K+ ATPase活性之间未发现显著的相关性。以上结果说明: 断奶前后仔猪H+ K+ ATPase的mRNA相对含量和活性没有明显的发育性变化, 断奶对H+ K+ ATPase mRNA表达和活性没有影响。

肝门阻断再灌注后脑钠素和心肌细胞膜Na^+-K^+ ATPase活性的改变

目的观察肝门阻断再灌注后血流动力学和心肌能量代谢改变。方法大鼠气管切开机械通气。随机分为假手术对照组(A组,n=24):不作肝血流的阻断;肝血流阻断组(B组,n=24):阻断肝十二指肠韧带60min后开放再灌注;门静脉转流下肝血流阻断组(C组,n=24):分别阻断肝左中叶及右叶肝蒂,保留尾叶血供作为门静脉血液回流通道,60min后再灌注。每组各有8只大鼠分别于再灌注前、再灌注后1、6h取材。血气分析研究肝门阻断期间门脉中pH值和电解质变化、ELISA检测脑钠素(BNP)水平以及比色法测定心肌细胞膜Na+-K+ATPase活性。结果与A组比较,B组再灌注前pH值显著降低,K+升高幅超过1倍(P<0.01),再灌注后开始下降,Ca2+也进行性下降;同时再灌注后B组肺动脉压(PAP)显著升高,6h后仍不能恢复;B组BNP再灌注后高于A组(P<0.05),但组内比较差异无统计学意义;再灌注后B组心肌Na+-K+ATPase活性显著降低(P<0.01)。结论肝门阻断后再灌注可引起脑钠素和心肌细胞膜Na+-K+ATPase活性改变。

甘草三参合剂对大鼠心肌细胞跨膜电位及Na^+-K^+ ATPase活性的影响

目的:探讨甘草三参合剂抗心律失常的作用机理。方法:大鼠连续灌药7d,造心肌缺血再灌注损伤动物模型,采用浮置式玻璃微电极引导左心室肌细胞跨膜电位(TMP),取缺血区心肌组织检测Na+K+ATPase活性。结果:甘草三参合剂能改善TMP幅度和时程,提高Na+K+ATPase活性,与模型组比较有显著差异(P<0.05),与阳性对照组心律平比较无显著差异(P>0.05)。结论:甘草三参合剂抗心律失常的作用机理可能是通过调节心肌细胞膜的Na+K+ATPase活性而影响跨膜电位、稳定心律的。

旱黑口服液对衰老小鼠心、脑细胞膜Na^+-K^+-ATPase、Ca^(2+)-Mg^(2+)-ATPase活性的影响

目的观察旱黑口服液对D-gal衰老小鼠心肌细胞膜、脑细胞膜上Na+-K+-ATP,ase、Ca2+-Mg2+-ATPase活性的影响,探讨旱黑口服液在延缓衰老方面的效应机制。方法以D-gal致亚急性衰老小鼠为模型,同时给予旱黑口服液治疗,6周后测定心、脑细胞膜上Na+-K+-ATPase、Ca2+-ATPase活性。结果与空白组比较,衰老组心、脑细胞膜上Na+-K+-ATPase、Ca2+-Mg2+-ATPase活性降低,经旱黑口服液治疗后心、脑细胞膜上Na+-K+-ATPase、Ca2+-Mg2+-ATPase活性活性明显提高。结论旱黑口服液具有提高D-gal致衰老小鼠心、脑细胞膜上Na+-K+-ATPase、Ca2+-Mg2+-ATPase活性,延缓衰老的作用。

肠缺血再灌注Na^＋-K^＋ATPase的变化及绞股蓝总皂甙对它的影响

18只家兔随机分为三组，假手术（SO）组：只行相应的手术等操作，未阴断肠系膜前动脉；缺血再灌注（IR）组，肠缺血90min，再灌注120min，绞肠蓝总皂甙（GP）组，缺血再灌注过程同IR组，但在再灌注开始时，同时静脉注射GP100mg/kg,再灌注 注120min时，分别取各组活体空肠2cm，冰冻保存，各测肠组织中Na^+-K^+ATPase活性，结果：Na^+-K^+ATPase活性IR组景低，GP组离干IR组（P＜0.05),接近于SO组（P＞0.05），结果提示肠缺血再灌注Na^+-K^+ATPase活性受抑制，而GP则能起到保护该酶的作用。

耐低钾水稻的根质膜ATPase和H^+分泌特性

对耐低钾和不耐低钾的水稻（ＯｒｙｚａｓａｔｉｖａＬ．）“威优４９”和“远诱１号”的根原生质膜ＡＴＰａｓｅ性质的研究表明，这两种水稻的质膜ＡＴＰａｓｅ活性的最适ｐＨ均为６０，均在底物ＡＴＰ浓度为３ｍｍｏｌ／Ｌ时达到最大反应速度，Ｋｍ值均在０．８５左右。Ｋ＋对这两种水稻的质膜ＡＴＰａｓｅ活性均具有促进作用。当介质中［Ｋｍ］≤５０ｍｍｏｌ／Ｌ时随［Ｋ＋］的增大，对耐低钾品种根质膜ＡＴＰａｓｅ活性的促进作用明显大于不耐低钾品种；当介质［Ｋ＋］在１００～２００ｍｍｏｌ／Ｌ之间时，Ｋ＋对两种水稻品种质膜ＡＴＰａｓｅ活性的刺激效应的差别减小。这两个水稻品种的基础Ｈ＋分泌没有明显差别，但钾刺激的Ｈ＋分泌存在差异，Ｋ＋对耐低钾品种Ｈ＋分泌的刺激效应大于不耐低钾品种。抑制剂实验表明在耐低钾和不耐低钾的水稻品种中，Ｋ＋刺激的根质膜ＡＴＰａｓｅ活性，Ｋ＋刺激的Ｈ＋分泌和Ｋ＋吸收之间存在着紧密的联系。对Ｋ＋刺激的质膜ＡＴＰａｓｅ活性和Ｈ＋分泌的抑制会减少根对Ｋ＋的吸收量。推测耐低钾水稻的质膜ＡＴＰａｓｅ和Ｈ＋分泌对Ｋ＋更为敏感，特别是在低浓度Ｋ＋存在时，可能是耐低钾水稻更能利用低浓度Ｋ＋、在低钾环境中能更好生长的一个原因。

Changes in soluble interleukin-2 receptor level in serum and Na^+ -K^+ -exchanging ATPase activity in semen of infertile men caused by antisperm antibody

Aim: To explore the possible mechanisms of male infertility caused by antisperm antibody (AsAb). Methods: Thesoluble interleukin-2 receptor (sIL-2R) level in serum was analyzed by ELISA and Na^+ -K^+ -exchanging ATPase activi-ty in semen by phosphorus (Pi) assay. Results: The slL-2R level in serum was significantly higher and the Na^+ -K^+ -exchanging ATPase activity in semen significantly lower in AsAb positive infertile men when compared with thecontrols. Conclusion: The AsAb titer varies with the slL-2R level in serum. A decrease in Na^+ -K^+ -exchangingATPase activity in semen may play a role in male infertility caused by AsAb.

Glutamate dehydrogenase and Na^+-K^+ ATPase expression and growth response of Litopenaeus vannamei to different salinities and dietary protein levels

Improvement in the osmoregulation capacity via nutritional supplies is vitally important in shrimp aquaculture.The effects of dietary protein levels on the osmoregulation capacity of the Pacific white shrimp(L.vannamei) were investigated.This involved an examination of growth performance,glutamate dehydrogenase(GDH) and Na+-K+ ATPase mRNA expression,,and GDH activity in muscles and gills.Three experimental diets were formulated,containing 25%,40%,and 50% dietary protein,and fed to the shrimp at a salinity of 25.After 20 days,no significant difference was observed in weight gain,though GDH and Na+-K+ ATPase gene expression and GDH activity increased with higher dietary protein levels.Subsequently,shrimp fed diets with 25% and 50% dietary protein were transferred into tanks with salinities of 38 and 5,respectively,and sampled at weeks 1 and 2.Shrimp fed with 40% protein at 25 in salinity(optimal conditions) were used as a control.Regardless of the salinities,shrimp fed with 50% dietary protein had significantly higher growth performance than other diets;no significant differences were found in comparison with the control.Shrimp fed with 25% dietary protein and maintained at salinities of 38 and 5 had significantly lower weight gain values after 2 weeks.Ambient salinity change also stimulated the hepatosomatic index,which increased in the first week and then recovered to a relatively normal level,as in the control,after 2 weeks.These findings indicate that in white shrimp,the specific protein nutrient and energy demands related to ambient salinity change are associated with protein metabolism.Increased dietary protein level could improve the osmoregulation capacity of L.vannamei with more energy resources allocated to GDH activity and expression.

应激状态下大鼠胃壁细胞H^+-K^+-ATP酶活性测定及电镜酶细胞化学研究

目的:探讨应激状态下大鼠胃壁细胞H+-K+-ATP酶活性及电镜酶细胞化学染色的变化。方法:将24只SD大鼠随机分为对照组、应激组和应激+奥美拉唑(OM)组,采用水浸-束缚应激(WRS)动物模型,检测胃粘膜溃疡指数(UI)和壁细胞H+-K+-ATP酶活性,观察壁细胞超微结构变化及H+-K+-ATP酶细胞化学染色结果。结果:应激组胃粘膜UI和壁细胞H+-K+-ATP酶活性明显高于对照组(P<0.01和P<0.05),而应激+OM组UI和H+-K+-ATP酶活性明显低于应激组(P<0.01);电镜下对照组壁细胞呈静息状态,应激组壁细胞内分泌小管密集呈激活状态,而应激+OM组分泌小管明显扩张,绒毛稀少;酶细胞化学染色显示对照组壁细胞的分泌小管和顶部质膜有少量黑色点状酶反应产物沉积,应激组壁细胞的分泌小管可见多量的、密集分布的黑色点状酶反应产物,而应激+OM组分泌小管上几乎无反应产物沉积。结论:应激状态下大鼠胃壁细胞H+-K+-ATP酶活性升高,且与壁细胞超微结构改变相一致,提示胃酸是应激性溃疡发生的重要因素之一。

幽门螺杆菌急性感染对胃壁细胞及H^+-K^+ATP酶mRNA基因表达的影响

目的 利用人类幽门螺杆菌急性感染的小鼠模型研究Hp对胃壁细胞及H + K +ATP酶mRNA基因表达的影响。方法 2 0只SPF级BALB/C小鼠分为两组 ,实验组和对照组 ,实验组动物每只灌胃 0 .4mlHp菌液 ,连续 5d ;而对照组予生理盐水灌胃。 2周后处死动物 ,取胃黏膜分别用于尿素酶试验、Giemsa染色 ;电镜观察壁细胞形态 ,用图象分析软件分别计算出两组分泌小管面积分数 ;用RT PCR测定H+ K+ ATP酶mRNA基因表达的情况。结果 实验组动物胃黏膜尿素酶试验及Giemsa染色均为阳性 ;图象分析软件结果显示分泌小管面积分数 ,试验组为 1.96± 0 .0 8/ 10 4 ,对照组为 4.2 9± 2 .30 / 10 4 ,两组比较有显著性差异 ;用RT PCR测定H+ K+ ATP酶mRNA基因表达结果显示实验组为 0 .92± 0 .14,对照组为 1.0 4± 0 .14,两组比较有显著性差异。结论 幽门螺杆菌急性感染后 ,胃酸分泌明显减少 ,减少的原因考虑与下调H+ K+

胃壁细胞H^+-K^+ATP酶mRNA基因表达的影响因素

促胃酸分泌因子、Hp感染及常用抑酸药物均可对H^+-K^+ATP酶mRNA基因表达产生影响;H^+-K^+ATP酶mRNA的改变继而可引起H^+-K^+ATP酶活性及壁细胞泌酸功能改变。

奥曲肽联合酚磺乙胺治疗上消化道出血的临床疗效及其对H^(+)-K^(+)-ATP酶活性的影响

目的探讨奥曲肽联合酚磺乙胺治疗上消化道出血的临床疗效及其对氢-钾离子-三磷酸酰胺酶(H^(+)-K^(+)-ATP酶)活性的影响。方法选取2020年1月-2021年6月井冈山市第二人民医院收治的上消化道出血患者60例,按照随机数字表法分为对照组(n=30)与观察组(n=30)。对照组予以酚磺乙胺注射液,观察组在对照组治疗基础上予以奥曲肽注射液,2组均持续治疗5 d。比较2组主要症状(呕血、腹痛、发热、黑便)消失时间,治疗前及治疗5 d后凝血功能指标[凝血酶原时间(PT)、活化部分凝血活酶时间(APTT)、凝血酶时间(TT)、纤维蛋白稳定因子(FSF)、纤维蛋白原(Fib)]、血液指标[血小板计数(PLT)、血细胞比容(HCT)]、H^(+)-K^(+)-ATP酶,并观察2组药物不良反应发生情况。结果观察组患者呕血、腹痛、发热、黑便消失时间短于对照组(P<0.05)。治疗5 d后,2组患者PT、APTT、TT短于治疗前,FSF、Fib高于治疗前,且观察组患者PT、APTT、TT短于对照组,FSF、Fib高于对照组(P<0.01)。治疗5 d后,2组患者PLT、HCT高于治疗前,H^(+)-K^(+)-ATP酶低于治疗前,且观察组患者PLT、HCT高于对照组,H^(+)-K^(+)-ATP酶低于对照组(P<0.01)。观察组患者不良反应总发生率为16.67%,与对照组的10.00%比较,差异无统计学意义(χ^(2)=0.144,P=0.704)。结论奥曲肽联合酚磺乙胺治疗上消化道出血的临床疗效确切,可快速缓解患者的临床症状,有效改善凝血功能,抑制H^(+)-K^(+)-ATP酶活性,且安全性较高。