Ca~(2 )-Calmodulin is Involved in Betacyanin Accumulation Induced by Dark in C_3 Halophyte Suaeda salsa

The C_3 halophyte Suaeda salsa was used to investigate the roles of Ca~(2 ),Ca~(2 )channels,and calmodulin(CAM)in betacyaninmetabolism.Seeds of S.salsa were cultured in both the dark and light for 3 days.The fresh weight and betacyanin contentwere much higher in S.salsa seedlings formed in the dark than in seedlings formed in the light.The addition of Ca~(2 )tothe half-strength MS nutrient solution promoted betacyanin accumulation in the dark,whereas Ca~(2 )depletion by EGTAsuppressed the dark-induced betacyanin accumulation in shoots of S.salsa.The Ca~(2 )channel blocker LaCl_3 also inhibiteddark-induced betacyanin accumulation.The highest activity of CaM and the maximum betacyanin content decreased by51% and 45%,respectively,in shoots of S.salsa seedlings treated with the potent CaM antagonist chlorpromazine in thedark.Furthermore,the other CaM antagonist N-(6-aminohexyl)-5-chloro-1-naphthalenesulfonamide(W-7)also inhibited theactivity of CaM and dark-dependent betacyanin accumulation,whereas its less active structural analog N-(6-aminohexyl)-1-naphthalenesulfonamide(W-5)had little effect on the responses to dark of S.salsa seedlings.These results suggest thatCa~(2 ),Ca~(2 )-regulated ion channels,and CaM play an important role in dark-induced betacyanin accumulation in the shootsof the C_3 halophyte S.salsa.     

白芷培养细胞外钙调素结合蛋白的胶体金电镜定位研究

利用胶体金标记技术制备了具有生物活性的植物CaM-BSA-gold探针,并用此探针建立了白芷愈伤组织培养细胞胞外钙调素结合蛋白(CaMBPs)的透射电镜标记方法。标记结果显示,在1mmol/L Ca~(2 )存在下,用EGTA洗涤过的白芷愈伤组织培养细胞壁表面有金颗粒分布,而分别在含有EGTA、TFP、过量未标记的CaM、CaM抗体存在的情况下,用金标CaM探针进行标记.以及用金标羊抗兔抗体替代金标CaM探针进行标记的各对照组,细胞壁表面金颗粒则消失,说明白芷愈伤组织培养细胞壁表面存在着CaM结合位点或CaMBPs。     

大麦与白粉病菌互作中钙调素的细胞化学定位

对不同抗病性的大麦近等基因系受白粉病菌侵染诱导后的钙调素(CaM)变化进行了免疫细胞化学研究。结果表明,钙调素普遍存在于各种不同类型的细胞中,代谢活跃的细胞中CaM标记密度相对较高;CaM分布于细胞核、细胞壁、叶绿体等细胞器中,其中细胞核标记密度最高。在健康叶片中,感病品系Ingrid伴胞中CaM的标记密度明显高于抗病品系mlo—3,而其他细胞中CaM标记密度没有明显差别。病原菌接种后,各种细胞的CaM标记密度均呈现一定程度的上升,但Ingrid上升幅度相对较大。在叶肉细胞中,mlo-3细胞核中CaM增加最明显。并对叶肉细胞和伴胞中CaM的变化进行了讨论。     

CaMBP-10单克隆抗体的制备及CaMBP-10在豌豆器官中的表达检测

用电泳纯钙调素结合蛋白BP 10 (CaMBP 10 )免疫小鼠 ,制备单克隆抗体 (McAb) .用MEP(mercapto ethtyl pyridine)HyperCel疏水层析柱从细胞培养上清中纯化并获得单克隆抗体 ,同时测定了抗体 抗原反应的基本特性 .此单克隆抗体具有较高纯度、特异性和亲和力 .亲和常数 (Kaff)为1 2 6× 10 9(mol L) -1,此抗体和CaM在空间上以相同或相近的位点与CaMBP 10相结合 .以胶体金标记的抗体为探针 ,研究CaMBP 10在豌豆幼叶、成熟叶、茎尖、茎、根等不同器官的分布特征 ,并与胶体金标记CaM的结合情况相对照 .结果显示 ,CaMBP 10在植物中的分布特点与文献报道的CaM的分布特点相一致 ,提示CaMBP 10可能是在蛋白水平上对CaM进行区域化和可用性调节     

小檗胺衍生物（EBB）体外抑制肺癌细胞增殖机制的初探

本文研究并发现了新型半天然钙调素(CaM)拮抗剂--O-4-乙氧基丁基小檗胺(O-4-ethoxy-butyl-berbamine,EBB),具有选择性抑制肺巨细胞癌(PG)的增殖和降低细胞内CaM水平的能力,对人胚肺细胞(HEL)的增殖和细胞内CaM的水平影响较小.同时观察到EBB引起肿瘤细胞内CaM水平降低的原因,是对CaM基因的转录产物(mRNA)和翻译产物(CaM)两方面作用的结果.此外,EBB还能部分降低PG细胞内原癌基因和突变的抑癌基因转录产物mRNA的水平.EBB抑制肿瘤细胞增殖的机制,除了对CaM基因的表达水平和CaM活性调控外,可能还直接或间接地影响了相关的原癌基因和突变的抑癌基因的表达.     

肌球蛋白轻链激酶CaM结合位点突变体的构建

目的:平滑肌肌球蛋白轻链激酶(myosin light chainkinase,MLCK)具有激酶活性和非激酶活性,在平滑肌收缩过程中起着关键酶调控的作用.为探寻MLCK的非激酶活性区域对MLCK活性的影响,本实验利用分子生物学技术构建了肌球蛋白轻链激酶CaM结合位点突变体,并纯化出重组的MLCK表达的蛋白质,为深入研究MLCK的非激酶活性在调节平滑肌收缩过程中的分子机制提供了实验基础.方法:利用野生型MLCK全长的cDNA序列设计CaM结合位点的突变引物,利用PCR技术进行定点突变,获得CaM结合位点的突变体(△CaM/MLCK).在大肠杆茵中表达重组CaM结合位点的突变体(△CaM/MLCK),通过亲和层析及凝胶过滤进行分离纯化重组蛋白,SDS-PAGE检测表达及纯化的重组蛋白.结果:构建重组MLCK钙调蛋白结合位点突变体(△CaM/MLCK),△CaM/MLCK在大肠杆菌中以可溶形式大量表达并得到纯化.结论:成功构建重组MLCK钙调蛋白结合位点突变体(△CaM/MLCK)并获得纯化的表达蛋白质.     

钙调素及其结合蛋白BP-10对类囊体膜蛋白磷酸化的作用

报道光诱导的内源类囊体膜蛋白的磷酸化可被一种新的植物钙调素(Calmodulin ,CaM )结合蛋白BP 1 0 (CaMBP -1 0 )显著抑制 ,并且抑制作用能被外加CaM消除 .同时 ,此磷酸化反应也可被EGTA和CaM拮抗剂TFP(trifluoperazine)及W 7(N ( 6 aminohexyl) -5- chloro -1 naphthalenesulfonamide)抑制 .提示 :( 1 )Ca ²⁺和CaM可能参与并调节植物光合作用 ;( 2 )催化类囊体膜蛋白磷酸化的激酶可能受Ca ²⁺和CaM调控 .进一步实验表明BP -1 0对类囊体膜蛋白的脱磷酸化作用无任何影响 .     

钙调蛋白的分布

钙调蛋白(Calmodulin.简写CaM),自从作为磷酸二酯酶的Ca~(2+)依赖性激活蛋白,被发现以来.现在已清楚CaM还是各种Ca~(2+)依赖性酶系的激活因子。据报道,在哺乳动物的各种组织以及蛙卵、章鱼、海胆卵、蚯蚓、扇贝、海葵、海蕈、藻类、霉菌、粘菌、四膜虫、大麦、人参、大豆、菠菜中都分离到了CaM或类CaM蛋白。显然CaM的广泛分布和作用是与其特有的多功能性分不开的。然而各种CaM的氨基酸组     

Ca^2＋-Calmodulin is Involved in Betacyanin Accumulation Induced by Dark in C3 Halophyte Suaeda salsa

The C3 halophyte Suaeda salsa was used to investigate the roles of Ca^2＋, Ca^2＋ channels, and calmodulin （CAM） in betacyanin metabolism. Seeds of S. salsa were cultured in both the dark and light for 3 days. The fresh weight and betacyanin content were much higher in S. salsa seedlings formed in the dark than in seedlings formed in the light. The addition of Ca^2＋ to the half-strength MS nutrient solution promoted betacyanin accumulation in the dark, whereas Ca^2＋ depletion by EGTA suppressed the dark-induced betacyanin accumulation in shoots of S. salsa. The Ca^2＋ channel blocker LaCl3 also inhibited dark-induced betacyanin accumulation. The highest activity of CaM and the maximum betacyanin content decreased by 51% and 45%, respectively, in shoots of S. salsa seedlings treated with the potent CaM antagonist chlorpromazine in the dark. Furthermore, the other CaM antagonist N-（6-aminohexyl）-5-chloro-l-naphthalenesulfonamide （W-7） also inhibited the activity of CaM and dark-dependent betacyanin accumulation, whereas its less active structural analog N-（6-aminohexyl）- 1-naphthalenesulfonamide （W-5） had little effect on the responses to dark of S. salsa seedlings. These results suggest that Ca^2＋, Ca^2＋-regulated ion channels, and CaM play an important role in dark-induced betacyanin accumulation in the shoots of the C3 halophyte S. salsa.     

化学发光法测定正常人皮肤纤维母细胞高密度脂蛋白(HDL)受体功能

A cbemiluminescence assay of human skin fibroblasts HDL receptor function was established.HDL3 was labelled with 6(N-(4-amino butyl)~N-ethyl)-amino-2,3-dihydro phthalazine l,4-dione(ABEI) by the carbodiimide(EDC).The labelled compound (HDL3-ABEI) was water soluble and non-toxic.It was stored at -30*********C before use.HDL3 was isolated by sequential ultracentrifugation.The HDL3 obtained was Apo-E-free.After incubation of HDL3 in waterbath at 52**********C for 3 hours, the HDL3 was labelled with ABEI to a ratio of 0.89 m mol ABEI/mmol HDL3.The HDL3-ABEI showed positive immunore action with antibodies of Apo A-********I and Apo A-*******II, indic-eting that the labelled HDL3 still retained its immunological characteristics.The conditions for determination of HDL receptor function of human skin fibroblasts were studied.The optimum quantity of HDL3-ABEI for combination with fibroblasts HDL receptors at 4癈 was 20********ug.The optimum time for combination of HDL3-ABEI with fibroblasts HDL receptors at 4*********C was 1 hour.The amount of HDL required for blocking HDL receptors was 400********ug.The optimum cell number for combination of HDL3-ABEI with HDL receptors was 1**********X105 cells/ml.In the mean time, the decrease in luminescence intensity with the increase in number of cells was observed.Again a high protein concentration would cause inhibition to the assay system.