共查询到19条相似文献,搜索用时 62 毫秒
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目的 :建立IgHV1抗原九肽荧光标记及分离纯化的方法。方法 :利用硫代磷酸化的原理以荧光试剂标记IgHV1抗原九肽 ,用葡聚糖凝胶 (Sephadex)G 1 5层析柱及聚丙烯酰胺凝胶电泳(PAGE)对荧光标记的IgHV1抗原九肽进行分离纯化并以毛细管电泳技术进行鉴定。结果 :用毛细管电泳技术对纯化后样品进行鉴定 ,其电泳图谱只出现单一峰。结论 :初步建立IgHV1抗原九肽荧光标记及分离纯化的方法 相似文献
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建立钐(Sm3+)标记检测C肽(C-peptide)及铕(Eu3+)标记检测胰岛素(insulin)的双标记时间分辨荧光免疫分析法(TRFIA),并初步尝试检测人血C肽以及胰岛素含量.将抗C肽单克隆抗体(Biodesign No.E54094M)与抗insulin单克隆抗体(BiodesignNo.E86306M)混合包被96孔板,然后用Sm3+标记抗C肽单克隆抗体(Medix No.9103),Eu3+标记抗insulin单克隆抗体(Biodesign No.E86802M),运用双抗体夹心一步法建立C肽/胰岛素双标记时间分辨免疫荧光分析法.结果显示:C肽分析灵敏度为0.2μg/L,线性范围为0.5~22μg/L,平均回收率达到99.6%,分析内和分析间变异系数分别为4.6%~6.0%和5.1%~7.6%.胰岛素分析灵敏度为0.8 mU/L,线性范围为3.6~180 mU/L,平均回收率为99.4%,分析内和分析间变异系数分别为3.7%~6.0%和5.1%~8.0%.C肽/胰岛素双标记检测试剂与PerkinElmer公司对应的单标记进口试剂盒分别同时测定血清样本200份,检测结果高度相关,具有较好的一致性,相关系数分别为0.98与0.99.总之,自建C肽/胰岛素双标记时间分辨荧光免疫分析方法的性能均可以达到临床检测要求,有望替代现有国内外较为昂贵的单标记试剂,可用于胰岛素分泌不足导致的糖尿病诊断及糖尿病的大规模普查筛选. 相似文献
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血浆激肽释放酶新底物PK┐120的研究蒲小平(军事医学科学院基础医学研究所,北京100850)关键词血浆激肽释放酶底物1.发现补体系统由20余种血浆蛋白组成,在机体防御和炎症应答反应中起重要作用。1989年Hammer等在用C4b-Sepharose... 相似文献
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利用噬菌体肽库筛选胰凝乳蛋白酶的底物 总被引:1,自引:0,他引:1
利用脱水胰凝乳蛋白酶 (保持天然酶的完整结合部位 ,但没有催化活性 )作为靶蛋白 ,在噬菌体肽库中钓取一些有结合活力噬菌体 ,再将得的噬菌体同固定化的天然酶一起保温 ,能够被天然酶水解的那部分噬菌体即为底物噬菌体 .利用 DNA测序技术测出筛得的短肽序列 ,分析序列保守性 ,发现 WR和 YF的组合具有很强的保守性 .合成相应的几个短肽 ,与天然酶作用 ,发现芳香族氨基酸与碱性氨基酸的组合较易被胰凝乳蛋白酶切割 .而且 ,当 P2 、P3 位置为侧链较小的氨基酸或碱性氨基酸时 ,更有利于水解的发生 .精氨酸无论处在任何位置 ,对水解往往都有促进作用 相似文献
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兔红细胞的荧光标记及寿命检测法 总被引:1,自引:0,他引:1
目的 :建立一种简单有效的兔红细胞标记及寿命检测法 ,并对GMA保养液 4℃保存的红细胞质量进行评价。方法 :日本大耳白兔动脉取血 ,红细胞用异硫氰酸荧光素 (FITC)标记后自体回输 ,定期检测荧光标记的红细胞数所占百分比。应用SAS软件对所得数据进行回归分析 ,根据方程计算兔体内标记红细胞的 2 4h回收率和半寿期。结果 :正常兔红细胞的 2 4h回收率是 93 .76%± 5.40 % ,半寿期为 ( 2 2 .50± 4.3 7)d ,与有关文献相符。GMA液 4℃保存 2 1d的红细胞 2 4h回收率为 89.13 %± 7.10 % ,半寿期为 ( 11.41± 1.63 )d ,符合输注条件。结论 :与其他红细胞体内标记方法相比 ,FITC标记法简便实用 ,价格便宜 ,不具有放射性危害 ,可用于输注红细胞的质量评价和体内生物学特性分析 相似文献
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荷包猪SLA-2重链基因偶合底物肽及表达研究 总被引:1,自引:0,他引:1
目的:构建荷包猪SLA-2重链基因偶合底物肽(BSP)并研究其在pET-21a(+)中的蛋白表达.方法:设计荷包猪SLA-2-BSP复合基因引物,PCR扩增荷包猪SLA-2-HB-BSP复合基因,并克隆至pMD(R)19-T Simple Vector,经酶切鉴定后,将SLA-2-HB-BSP复合基因与表达系统pET-21a(+)连接,并转化BL21 (Rosetta)菌进行诱导表达,SDS-PAGE检测目的蛋白.结果:PCR结果显示,SLA-2-BSP大小为900bp左右,并成功克隆至pMD(R)19-T Simple Vector载体,酶切后大小为876bp,该基因连接pET-21 a(+)并转化宿主菌BL21(Rosetta)后,经诱导表达和SDS-PAGE检测,目标蛋白大小为34.4kDa,经优化后目的蛋白相对表达含量达到了45%.结论:该研究成功构建荷包猪SLA-2偶合BSP的pET-21a重组表达系,为下一步构建猪SLA Ⅰ类分子四聚体奠定了基础. 相似文献
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通过 RT- PCR,从人肝组织中扩增出血管形成抑制素 ( angiostatin) c DNA的 K1片段 ,经DNA序列分析证实其正确性 ;将 K1与 GST融合并带上 1 7个氨基酸的 PKA底物磷酸化基序 ,IPTG诱导表达 ,以还原型谷胱甘肽偶联的琼脂糖凝胶亲合层析直接从细菌裂解上清中纯化融合蛋白 ;以 PKA催化单位将 3 2 P通过磷酸化作用标记至纯化的蛋白 ,再用凝血酶切去 GST,进行SDS- PAGE.放射自显影结果显示 ,GSTag- K1和 Tag- K1分别在 40 k D和 1 7k D处有信号强而特异的显影条带 ,表明带有磷酸化序列的蛋白能够被 PKA特异地磷酸化标记 相似文献
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促分裂原活化蛋白激酶磷酸酶 总被引:4,自引:0,他引:4
促分裂原活化蛋白激酶磷酸酶(mitogen-activated protein kinase phosphatases,MKPs)是一类丝/苏氨酸和酪氨酸双特异性的磷酸酶。它在细胞分化、增殖和基因表达过程中起着重要的作用。MKPs可以选择性地结合促分裂原活化蛋白激酶(mitogen-activated protein kinase,MAPK),对MAPK进行去磷酸化,从而调节MAPK信号通路的活性。另一方面,MAPK也可以激活MKPs,它们的相互作用确保了细胞内信号的精确传递,并参与细胞功能的调节。 相似文献
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酪氨酸蛋白激酶和蛋白激酶C对N-乙酰氨基葡萄糖转移酶V的双重调控 总被引:2,自引:0,他引:2
在人肝癌细胞7721中研究了酪氨酸蛋白激酶(TPK)和蛋白激酶C(PKC)的激活剂[分别为表皮生长因子(EGF)和佛波酯(PMA)]和各种蛋白激酶抑制剂对N-乙酰氨基葡萄糖转移酶V(GnT-V)活力的影响,以探讨TPK和PKC对GnT-V的调节。结果发现,EGF或PMA处理细胞48h后,GnT-V的活力明显增高;蛋白激酶的非特异性抑制剂槲皮素和染料木黄酮(genistein)在抑制TPK和PKC的同时,抑制GnT-V的基础活力,并完全阻断EGF或PMA对GnT-V的增高作用;TPK的特异性抑制剂Tyrphostin-25和PKC的特异性抑制剂D-鞘氨醇分别应用时,各自只能部分地取消EGF或PMA对GnT-V的诱导。但当Tyrphostin-25和D-鞘氨醇同时加入培养基中则可完全阻断EGF或PMA对GnT-V的诱导激活。蛋白质合成抑制剂环己亚胺和蛋白激酶抑制剂作用相仿,不但可抑制GnT-V的基础活力,也可完全消除EGF或PMA对GnT-V的激活。以上结果提示EGF或PMA通过蛋白激酶调节GnT-V的酶蛋白合成,并且GnT-V受到膜性TPK和PKC的双重调节,其中m-TPK较m-PKC更为重要。 相似文献
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为研究蛋白激酶C(protein kinase C,PKC)在小鼠早期发育中的调节作用,运用超排卵和体外受精技术,采用体外磷酸化和放射自显影的方法,鉴定小鼠1-细胞期受精卵中PKC的底物。经特殊的反复冻融处理,消除卵中内源性蛋白激酶活性。55个受精卵的样品中加入部分纯化的PKC,结合应用较强的PKC抑制剂H-7和星形孢菌素以及促分裂原活化蛋白激酶抑制剂PD098059作为对照,观察到12条PKC底物蛋白的放射自显影带,根据标准蛋白质对值绘制的标准曲线计算,这些磷酸化蛋白的相对分子量分别约为120kDa、100kDa、79kDa、63kDa、59kDa、47kDa、40kDa、34kDa、32kDa、26kDa、24kDa和22kDa。实验结果表明,PKC可通过底物蛋白活性的调节,在小鼠早期发育中发挥重要作用。 相似文献
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Crystal structures of the catalytic subunit α of cAMP-dependent protein kinase (PKAc) with three adenosine analogue-oligoarginine conjugates (ARCs) are presented. The rationally designed ARCs include moieties that, in combination, target both the ATP- and the peptide-substrate-binding sites of PKAc, thereby taking advantage of high-affinity binding interactions offered by the ATP site while utilizing an additional mechanism for target specificity via binding to the peptide substrate site. The crystal structuresdemonstrate that, in accord with the previously reported bisubstrate character of ARCs, the inhibitors occupy both binding sites of PKAc. Further, they show new binding modes that may also apply to natural protein substrates of PKAc, which have not been revealed by previous crystallographic studies. The crystal structures described here contribute to the understanding of the substrate-binding patterns of PKAc and should also facilitate the design of inhibitors targeting PKAc and related protein kinases. 相似文献
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Coordinated Regulation of Radioadaptive Response by Protein Kinase C and p38 Mitogen-Activated Protein Kinase 总被引:8,自引:0,他引:8
Takashi Shimizu Tomohisa Kato Jr. Akira Tachibana Masao S. Sasaki 《Experimental cell research》1999,251(2):424-432
Eukaryotic cells are known to have an inducible or adaptive response that enhances radioresistance after a low priming dose of radiation. This radioadaptive response seems to present a novel cellular defense mechanism. However, its molecular processing and signaling mechanisms are largely unknown. Here, we studied the role of protein kinase C (PKC) and mitogen-activated protein kinase (MAPK) in the expression of radioadaptive response in cultured mouse cells. Protein immunoblot analysis using isoform-specific antibodies showed an immediate activation of PKC-alpha upon X-irradiation as indicated by a translocation from cytosol to membrane. A low priming dose caused a prolonged translocation, while a nonadaptive high dose dramatically downregulated the total PKC level. Low-dose X-rays also activated the p38 MAPK. The activation of p38 MAPK and resistance to chromosome aberration formation were blocked by SB203580, an inhibitor of p38 MAPK, and Calphostin C, an inhibitor of PKC. Furthermore, it was demonstrated that p38 MAPK was physically associated with delta1 isoform of phospholipase C (PLC-delta1), which hydrolyzed phosphatidylinositol bisphosphate into diacylglycerol, an activator of PKC, and that SB203580 also blocked the activation of PKC-alpha. These results indicate the presence of a novel mechanism for coordinated regulation of adaptive response to low-dose X-rays by a nexus of PKC-alpha/p38 MAPK/PLC-delta1 circuitry feedback signaling pathway with its breakage operated by downregulation of labile PKC-alpha at high doses or excess stimuli. 相似文献
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Abstract: To determine whether protein kinase C (PKC) mediates release of peptides from sensory neurons, we examined the effects of altering PKC activity on resting and evoked release of substance P (SP) and calcitonin gene-related peptide (CGRP). Exposing rat sensory neurons in culture to 10 or 50 n M phorbol 12,13-dibutyrate (PDBu) significantly increased SP and CGRP release at least 10-fold above resting levels, whereas the inactive 4α-PDBu analogue at 100 n M had no effect on release. Furthermore, 100 n M bradykinin increased peptide release approximately fivefold. Down-regulation of PKC significantly attenuated the release of peptides evoked by either PDBu or bradykinin. PDBu at 1 n M or 1-oleoyl-2-acetyl- sn -glycerol at 50 µ M did not alter resting release of peptides, but augmented potassium- and capsaicin-stimulated release of both SP and CGRP approximately twofold. This sensitizing action of PKC activators on peptide release was significantly reduced by PKC down-regulation or by pretreating cultures with 10 n M staurosporine. These results establish that activation of PKC is important in the regulation of peptide release from sensory neurons. The PKC-induced enhancement of peptide release may be a mechanism underlying the neuronal sensitization that produces hyperalgesia. 相似文献
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Kaushal Parikh Sander H. Diks Jurriaan H. B. Tuynman Auke Verhaar Mark L?wenberg Daan W. Hommes Jos Joore Akhilesh Pandey Maikel P. Peppelenbosch 《PloS one》2009,4(7)
Kinases are pivotal regulators of cellular physiology. The human genome contains more than 500 putative kinases, which exert their action via the phosphorylation of specific substrates. The determinants of this specificity are still only partly understood and as a consequence it is difficult to predict kinase substrate preferences from the primary structure, hampering the understanding of kinase function in physiology and prompting the development of technologies that allow easy assessment of kinase substrate consensus sequences. Hence, we decided to explore the usefulness of phosphorylation of peptide arrays comprising of 1176 different peptide substrates with recombinant kinases for determining kinase substrate preferences, based on the contribution of individual amino acids to total array phosphorylation. Employing this technology, we were able to determine the consensus peptide sequences for substrates of both c-Raf and Mitogen Activated Protein Kinase Kinase Kinase 8, two highly homologous kinases with distinct signalling roles in cellular physiology. The results show that although consensus sequences for these two kinases identified through our analysis share important chemical similarities, there is still some sequence specificity that could explain the different biological action of the two enzymes. Thus peptide arrays are a useful instrument for deducing substrate consensus sequences and highly homologous kinases can differ in their requirement for phosphorylation events. 相似文献
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用增强绿色荧光蛋白特异性标记小鼠 3T3 L1前脂肪细胞系 .构建paP2 promoter EGFP载体 ,电穿孔转染小鼠 3T3 L1前脂肪细胞 ,显微荧光观察和RT PCR确认aP2基因的内源表达 .EGFP基因转入 3T3 L1前脂肪细胞 ,观察到细胞分化过程中EGFP表达和脂肪积累 .RT PCR分析表明 ,EGFP代表了稳定而真实的aP2基因的内源性表达 .建立了由脂肪组织特异表达基因aP2的表达控制的EGFP标记的小鼠 3T3 L1前脂肪细胞系 ,目前尚未见用同样方法对前脂肪细胞进行特异性标记 .该细胞系将为脂肪细胞分化机理研究以及为抗肥胖症和抗糖尿病药物筛选提供有力工具 . 相似文献
