灵芝肽多糖生物活性初探

从人工培养的灵芝菌丝体中分离纯化得到灵芝肽多糖(简称GPP)。经测定,GPP分子量为140000,单糖组成为木糖、葡萄糖、半乳糖及半乳糖醛酸。GPP分子中含蛋氨酸、赖氨酸等13种氨基酸。动物实验表明,GPP能显著提高小鼠腹腔吞噬细胞的吞噬能力,增强体液免疫和红细胞免疫功能,并能提高红细胞中超氧化物岐化酶(SOD)的活性。

抗肿瘤活性青蛤多肽的提取工艺研究

[目的]探究具有抗肿瘤活性的青蛤多肽的最佳提取工艺路线.[方法]选择胰蛋白酶酶解青蛤,以酶解液对PC-3细胞增殖抑制率（IR）为指标,研究料液比、温度、pH、加酶量和酶解时间对多肽提取率的影响,探讨最佳工艺,并采用超滤及G25洗脱分离纯化提取液.[结果]当温度为45℃、pH为7.0、料液比为1∶3、酶解时间为6h、加酶量为300 U/g时,分子量为3～5 kD青蛤提取液的抗肿瘤活性最好;分离纯化后在280 nm波长处得到3个峰,其中峰1和峰2成分抗肿瘤活性显著.[结论]以细胞增殖抑制率为指标可以确定青蛤多肽的提取及优化工艺路线.

肾上腺髓质素原N端20肽对血管紧张素刺激心肌成纤维细胞生成NO的影响

目的探讨肾上腺髓质素原N端20肽(PAMP)对血管紧张素II刺激心肌成纤维细胞(CFs)生成NO的影响及意义。方法采用胰酶消化、差速贴壁法培养新生SD大鼠CFs,以硝酸还原法测定细胞培养液中NO的浓度,分别观察不同浓度AngII、PAMP、及AngII+PAMP对CFs生成NO的影响。结果(1)10-9、10-8、10-7、10-6μmol/LAngII组细胞培养液中的浓度是:(73.88±2.23)、(64.34±3.02)、(54.12±2.82)、(40.21±1.45)μmol/L,各组之间有显著性差异(P<0.01)。(2)10-9、10-8、10-7、10-6μmol/LPAMP组细胞培养液中NO的浓度分别为(74.40±3.42)、(74.91±2.66)、(75.77±3.31)、(74.23±2.43)μmol/L,而空白组为(74.57±2.49)μmol/L。各组之间无显著性差异(P>0.05)。(3)10-7μmol/LAngII+(10-9、10-8、10-7、10-6μmol/L)PAMP组培养液中NO合成浓度分别为(66.15±2.95)、(80.58±3.77)、(88.67±1.46)、(96.22±2.96)μmol/L,各组间有显著性差异(P<0.01)。结论随AngⅡ浓度增加可显著抑制CFs分泌NO,而PAMP对CFS合成NO无明显影响,但PAMP与AngII共同培养时,随PMAP浓度增加,NO的合成呈依从性增多。

Expression of CTB-human Insulin(BA) Fusion Protein in Gynostemma Pentapyhllum Makino Callus Cells and Its Hypoglycemic Effect in Mice

The plant expression vector of choleratoxin B subunit（CTB）-human insulin（BA） fusion protein pBI121/（CTB-BA） was constructed first and then the Gynostemma Pentapyhllum Makino callus cell line that could express CTB-human insulin fusion protein was constructed and its hypoglycemic effect was evaluated in mice. The plant expression vector pBl 121/（CTB-BA） was digested with both BamI and SacI. Agrobacterium tumerfaciens strain LBA4404 was transformed with previously constructed recombinant plasmid pBI121/（CTB-BA） via the freeze thawing method, then CTB-BA gene was integrated to G Pentapyhllum Makino callus cells by co-culturing the cells with the transformed LBA4404 strain. The transformed G Pentapyhllum Makino callus cells were identified by DNA sequence assey and RT-PCR. The expressed product was identified by western-blot and its amount was tested by ELISA kit and its blood sugar decreasing effect was tested in mice. The sequences of synthetic CTB and human insulin genes（BA） were completely identical to those designed. Restriction map proved that the length of gene fragment in- serted into expression vector pBI121 was consistent with that expected. The sequence of genomic DNA of expressed product was completely identical to that designed. The result of RT-PCR was consistent with that expected. The expressed product showed a specific band with a relative molecular mass of 17000 by Western-blot. The human insulin expression amount was 6.03 μIU/mL according to the ELISA result. The animal test showed that only the G Pentapyhllum Makino callus cell line itself showed activity in decreasing the blood sugar of mice, however, the activity of the transformed G Pentapyhllum Makino callus cells was much higher, The plant expression vector pBI121/（CTB-BA） was constructed and expressed in the G Pentapyhllum Makino callus cells successfully for the first time. The trans- formed G Pentapyhllum Makino callus cells showed high activity in decreasing the blood sugar of mice. This study developed a new way for the development of oral administration insulin.

脑钠肽治疗肺栓塞的临床效果及对肺动脉收缩压和Tei指数的影响

目的观察脑钠肽(BNP)治疗肺栓塞(PE)的疗效。方法 82例肺栓塞患者随机分为脑钠肽组和对照组,每组41例。脑钠肽组在常规治疗基础上加用脑钠肽治疗,对照组采用常规治疗。观察两组临床疗效,测定两组治疗前后肺动脉收缩压和Tei指数。结果脑钠肽组总有效率为90.2%。高于对照组68.3%(P<0.05);治疗后,脑钠肽组的肺动脉收缩压和Tei指数均低于对照组[(21±10)vs(35±11)mmHg,(0.37±0.09)vs(0.64±0.05),P<0.01]。结论脑钠肽对肺栓塞患者疗效显著,能显著降低PE患者的肺动脉收缩压和Tei指数。

血浆ET和CGRP与高血压左室肥厚的关系研究现状

目的:探讨高血压左室肥厚与血浆ET和CGRP的关系的研究现状。方法:阅读国内外大量相关文献,加以归纳总结,得出结论。结果:血浆ET可能是一种促高血压左室肥厚因子,CGRP可能是一种抗高血压左室肥厚因子。结论:左室肥厚是高血压病人左室重构的重要表现,是发生心、脑血管事件的一个独立危险因素,逆转LVH成为抗高血压治疗的重要目标,通过某种途径使血浆ET浓度下降和CGRP浓度的升高,可能有助于高血压与高血压左室肥厚的治疗。

非糖尿病急性心肌梗死合并应激性高血糖患者血浆脑钠肽水平变化

目的探讨血浆脑钠肽(BNP)水平在非糖尿病急性心肌梗死(AMI)合并应激性高血糖患者病情评估中的作用。方法将我院2010年1月至11月收治的AMI患者60例患者根据空腹血糖值分为两组,非糖尿病AMI合并应激性高血糖组(试验组)36例(血糖≥7.0 mmol/L),AMI未合并应激性高血糖组(对照组)24例(血糖<7.0 mmol/L),在发病后24 h行血浆BNP浓度检测。结果发病后24 h血浆BNP水平在非糖尿病AMI合并应激性高血糖组明显高于AMI未合并应激性高血糖组[(671.87±631.71)ng/L vs(299.53±455.67)ng/L,P<0.01]。结论血浆BNP水平可以判断非糖尿病AMI合并应激性高血糖患者病情危重程度。

左西孟旦对扩张型心肌病失代偿患者N末端B型脑钠肽前体及心功能的影响

目的探讨左西孟旦治疗扩张型心肌病(DCM)失代偿患者血浆N末端B型脑钠肽前体(NT-proBNP)表达变化及心功能的影响。方法 56例DCM失代偿患者,随机分为对照组(31例)和治疗组(25例)。对照组采用常规治疗,治疗组在常规治疗基础上加用左西孟旦治疗,比较两组疗效。结果治疗组患者有效23例,有效率为92.0%,对照组患者有效27例,有效率为87.1%,两组有效率比较差异无统计学意义(χ~2=0.348,P>0.05)。治疗后,治疗组NT-proBNP浓度显著低于对照组,左心室射血分数(LVEF)高于对照组,差异具有统计学意义(P<0.05),两组左室舒张末内径比较,差异无统计学意义(P>0.05)。结论左西孟旦可有效改善DCM失代偿患者症状,进一步降低患者血浆NT-proBNP浓度和改善心脏收缩功能,值得借鉴。

降钙素基因相关肽对脂多糖诱导的巨噬细胞表达髓样细胞触发受体-1的影响(英文)

目的:探讨降钙素基因相关肽(CGRP)对脂多糖(LPS)诱导的小鼠巨噬细胞表达髓样细胞触发受体-1(TREM-1)的影响及其信号转导途径。方法:采用反转录-聚合酶链式反应(RT-PCR)观察巨噬细胞TREM-1mRNA表达量的变化,应用流式细胞术检测巨噬细胞膜表面TREM-1蛋白的表达。结果:CGRP对未受刺激的巨噬细胞表达TREM-1无明显影响,LPS可诱导巨噬细胞表达TREM-1;CGRP预处理呈剂量和时间依赖性上调LPS所致的巨噬细胞TREM-1mRNA的表达;同时,CGRP上调LPS所致的巨噬细胞膜表面TREM-1蛋白的表达;上述作用均可被PKC阻断剂H-7和PKA阻断剂H-89部分逆转(P<0.05)。结论:CGRP上调LPS诱导的巨噬细胞表达TREM-1,其胞内信号转导途径与PKA和PKC有关。

LCZ696在心血管疾病中的研究进展

LCZ696是第一个脑啡肽酶与血管紧张素受体联合阻滞的药物,脑啡肽酶能降解具有生物活性的利钠肽和其他几种血管活性物质,利钠肽具有排钠、舒张血管、阻断肾素-血管紧张素系统,降低交感张力、抗心肌细胞肥大等作用,脑啡肽酶阻滞剂可增加血浆利钠肽水平,而单独的脑啡肽酶阻滞剂并未带来临床获益,它需要与肾素-血管紧张素系统阻滞剂药物联用。多项临床研究表明,在高血压、心力衰竭的患者中使用LCZ696后,特别是在收缩性心力衰竭患者中,有显著的临床获益,现对LCZ696的机制及临床应用进展做一综述。

N端脑钠肽前体与维持性血液透析患者心血管疾病关系的研究进展

心血管疾病在维持性血液透析(MHD)患者中发生率较高,是其主要死因。N端脑钠肽前体(NT-proBNP)是由心室肌细胞合成和分泌的肽类激素,可以反映体内心肌细胞受到的容量负荷和压力负荷的大小,已广泛应用于正常人群的心血管疾病的诊断、治疗及预后评价。近年来大量研究证明,NT-proBNP也可作为监测MHD患者心血管疾病的重要生物学标志,其浓度对早期评判MHD患者心脏结构和功能异常、预测心血管事件发生及死亡、评估容量负荷等具有重要价值。

用人外周血淋巴细胞短期培养观察胎盘免疫调节肽的细胞遗传学效应

短期培养人外周血淋巴细胞的遗传效应实验表明,胎盘免疫调节肽不能显著诱发姐妹染色单体交换(P>0.05),不同剂量胎盘免疫调节肽组间姐妹染色单体交换频率也无显著差异(P>0.05),但在同等培养条件下,环磷酰胺能非常显著地使姐妹染色单体交换频率增高(P<0.001),提示胎盘免疫调节肽机体遗传物质的稳定性无影响。

Interaction of synthetic peptide corresponding to signal sequence of glucitol permease of Escherichia Coli and its analogue with liposomes

The N-terminal signal sequence of glucitol pcrmease of Escherichia Coli (Gut22) and its analogue (Gut22Ana) were synthesized. The analogue had a Pro residue substituting for the His at the 7th position of Gut22 and a Val residue substituting for the Glu at the 10th position. The intrinsic fluorescence emission spectra indicated that the binding of Gut22 with lipid bilayer was much stronger than that of Gut22Ana. The leakage experiments with calcein-loaded liposomes showed that Gut22 strongly perturbed lipid bilayers while Gut22Ana did not. The apparent partition constant of Gut22 for partitioning into phosphatidylserine/phosphatidylcholine bilayers was measured; the effect of membrane potential on the interaction of Gut22 with lipid bilayers was studied and the conformation changes of Gut22 and Gut22Ana upon interacting with liposomes were studied by the method of circular dichroism analysis.