蛋白质C

血液中的蛋白质C被激活后,通过多种方式促进凝血因子Xa和Ⅱa的形成．起到抗血液凝固、抗血栓形成的作用。蛋白质C功能异常,是一些血栓形成的原因。     

Molecular properties of phosphoenolpyruvate carboxylase from C3, C3−C4 intermediate,and C4 Flaveria species

Phosphoenolpyruvate carboxylase (PEPCase; EC 4.1.1.31) from Flaveria trinervia Mohr (C₄), F. floridana Johnston (C₃–C₄), and F. cronquistii Powell (C₃) leaves were compared by electrotransfer blotting/enzyme-linked immunoassay (Western-blot analysis), mobility of the native enzyme in polyacrylamide gels and in isoelectric focusing (IEF) gels, peptide mapping, and in-vitro translation of RNA isolated from each plant. The PEPCases from the C₃ and C₃–C₄ plants were very similar to each other in terms of electrophoretic mobilities on gels and isoenzyme patterns on IEF gels, and identical in peptide mapping. Quantitative differences were noted, however, in that the C₃–C₄ intermediate plant contained more PEPCase overall and that the relative activity of individual isoenzymes shifted between the C₃ and C₃–C₄ intermediate PEPCases. The PEPCase from the C₄ plant had a different isoenzyme pattern, a different peptide map, and was far more abundant than the other two enzymes. Western blot analysis demonstrated the cross-reactivity of PEPCases from all three Flaveria species with antibody raised against maize PEPCase. The results provide evidence, at the molecular level, that supports the view of C₃–C₄ intermediate species as C₃-like plants with some C₄-like photosynthetic characteristics, but there are differences from the C₃ plant in the quantity and properties of the PEPCase from the C₃–C₄ intermediate plant.Abbreviations IEF isoelectric focusing - kDa kilodalton - PEPCase phosphoenolpyruvate carboxylase - Rubisco Ribulose-1,5-bisphosphate carboxylase/oxygenase     

C3植物中C4途径的研究进展

综述了C3植物中C4途径的发现及研究现状;阐述了C3植物中C4途径的几种作用机理;根据C3植物中C4途径的存在,探讨了改造C3植物的遗传特性;并展望了这一领域的研究前景。     

C3植物中C4途径的研究进展

综述了Ｃ３植物中Ｃ４途径的发现及研究现状：阐述了Ｃ３植物中Ｃ４途径的几种作用机理;根据Ｃ３植物中Ｃ４途径的存在,探讨了改造Ｃ３植物的遗传特性;并展望了这一领域的研究前景。     

3C胰岛素泵

2012年5月19日,美敦力宣布722实时动态胰岛素泵系统在中国上市,这是国内首款3C整合系统的胰岛素泵。所谓3C整合系统,即同时实现实时动态血糖监测（CGM）、胰岛素持续输注（CSII）与糖尿病信息管理（CareLink）。     

如何快速鉴别C3与C4植物

在农业实践和科学研究中经常需要知道某种植物是C_3植物还是C_4植物,例如在干旱少雨的地区种植C_4作物就易获得较高的产量;用甲醇喷洒植物能使植物增产,但这种技术只适用于C_3植物而不适用于C_4植物等。从理论上讲,C_3植物光合作用固定CO_2的最初产物是三碳的3—磷酸甘油酸,C_4植物光合作用固定CO_2的最初产物是四碳的苹果酸或天冬氨酸。我们在研究农田杂草光合碳同化途径时,摸索了一些快速区分C_3植物与C_4植物的经验,介绍如下。 从植物进化方面区分 我们知道,C_3植物较原始,C_4植物较进化,实际上较原始的蕨类植物和裸子植物就没有C_4植物,只有较进化     

蛋白C,蛋白C激活剂和血栓性疾病

蛋白C(ProteinC,PC)系统是存在于人血浆中的天然抗凝系统,由蛋白C、蛋白S(PS)、血栓调节蛋白(TM)和蛋白C抑制剂(PCI)组成。许多研究结果表明:PC的病理改变与血栓性疾病的发生发展密切相关,PC可作为血栓性疾病诊断、疗效观察和预后评价的参考指标;PC和蛇毒PC激活剂有显著的抗凝溶栓效果,有应用于临床的可能性。现就这方面的进展作一简要综述。1　PC的生理功能和生物学特性　　PC是维生素K依赖性糖蛋白,以无活性的酶原形式存在于血浆中,由肝脏合成。PC是机体的一种重要的抗凝因子,约占血液抗凝活力的20%～30%,PC在微循环中的抗凝…     

C3、C4和C3-C4中间型植物的进化

介绍了有关C3、C4和C3-C4中间型植物进化的形态学、生理学、分子生物学、遗传学等方面的证据;推断地球上首先出现C3植物,然后是C3-C4中间类型植物,最后出现C4植物.     

C3和C4植物的氮素利用效率

Ｃ＿３和Ｃ＿４植物的氮素利用效率何新华,ＡｎｎＯａｋｓ,李明启（云南师范大学生物系,昆明６５００９２）（圭尔夫大学植物系,加拿大ＮＩＧ２Ｗ１）（华南农业大学农业生物系,广州５１０６４２）关键词Ｃ＿３和Ｃ＿４植物,ＮＯ吸收与积累,硝酸还原酶酶蛋白,硝酸...     

贺谈老百岁华诞

谈家桢教授是国际著名遗传学家,我国现代遗传学的奠基人之一,他也是一位卓越的教育家和社会活动家。 1909年9月15日,谈家桢先生出生于浙江宁波。他就读于苏州东吴大学,1930年获理学学士学位。随后赴北京燕京大学攻读硕士学位,导师是我国现代遗传学奠基人之一的李汝祺教授,1932年获硕士学位。经导师推荐,谈家桢先生赴美国深造,师从当代遗传学宗师摩尔根,在遗传学家杜布赞斯基的指导下完成博士研究生学业,于1936年获美国加州理工学院哲学博士学位。     

Complement components C5 and C7: recombinant factor I modules of C7 bind to the C345C domain of C5

Studies reported over 30 years ago revealed that latent, nonactivated C5 binds specifically and reversibly to C6 and C7. These reversible reactions are distinct from the essentially nonreversible associations with activated C5b that occur during assembly of the membrane attack complex, but they likely involve some, perhaps many, of the same molecular contacts. We recently reported that these reversible reactions are mediated by the C345C (NTR) domain at the C terminus of the C5 alpha-chain. Earlier work by others localized the complementary binding sites to a tryptic fragment of C6 composed entirely of two adjacent factor I modules (FIMs), and to a larger fragment of C7 composed of its homologous FIMs as well as two adjoining short consensus repeat modules. In this work, we expressed the tandem FIMs from C7 in bacteria. The mobility on SDS-polyacrylamide gels, lack of free sulfhydryl groups, and atypical circular dichroism spectrum of the recombinant product rC7-FIMs were all consistent with a native structure. Using surface plasmon resonance, we found that rC7-FIMs binds specifically to both C5 and the rC5-C345C domain with K(D) approximately 50 nM, and competes with C7 for binding to C5, as expected for an active domain. These results indicate that, like C6, the FIMs alone in C7 mediate reversible binding to C5. Based on available evidence, we suggest a model for an irreversible membrane attack complex assembly in which the C7 FIMs, but not those in C6, are bound to the C345C domain of C5 within the fully assembled complex.     

Co-function of C3-and C4-photosynthetic pathways in C3, C4 and C3-C4 intermediate Flaveria species

The potential for C₄ photosynthesis was investigated in five C₃-C₄ intermediate species, one C₃ species, and one C₄ species in the genus Flaveria, using ¹⁴CO₂ pulse-¹²CO₂ chase techniques and quantum-yield measurements. All five intermediate species were capable of incorporating ¹⁴CO₂ into the C₄ acids malate and aspartate, following an 8-s pulse. The proportion of ¹⁴C label in these C₄ products ranged from 50–55% to 20–26% in the C₃-C₄ intermediates F. floridana Johnston and F. linearis Lag. respectively. All of the intermediate species incorporated as much, or more, ¹⁴CO₂ into aspartate as into malate. Generally, about 5–15% of the initial label in these species appeared as other organic acids. There was variation in the capacity for C₄ photosynthesis among the intermediate species based on the apparent rate of conversion of ¹⁴C label from the C₄ cycle to the C₃ cycle. In intermediate species such as F. pubescens Rydb., F. ramosissima Klatt., and F. floridana we observed a substantial decrease in label of C₄-cycle products and an increase in percentage label in C₃-cycle products during chase periods with ¹²CO₂, although the rate of change was slower than in the C₄ species, F. palmeri. In these C₃-C₄ intermediates both sucrose and fumarate were predominant products after a 20-min chase period. In the C₃-C₄ intermediates, F. anomala Robinson and f. linearis we observed no significant decrease in the label of C₄-cycle products during a 3-min chase period and a slow turnover during a 20-min chase, indicating a lower level of functional integration between the C₄ and C₃ cycles in these species, relative to the other intermediates. Although F. cronquistii Powell was previously identified as a C₃ species, 7–18% of the initial label was in malate+aspartate. However, only 40–50% of this label was in the C-4 position, indicating C₄-acid formation as secondary products of photosynthesis in F. cronquistii. In 21% O₂, the absorbed quantum yields for CO₂ uptake (in mol CO₂·[mol quanta]^-1) averaged 0.053 in F. cronquistii (C₃), 0.051 in F. trinervia (Spreng.) Mohr (C₄), 0.052 in F. ramosissima (C₃-C₄), 0.051 in F. anomala (C₃-C₄), 0.050 in F. linearis (C₃-C₄), 0.046 in F. floridana (C₃-C₄), and 0.044 in F. pubescens (C₃-C₄). In 2% O₂ an enhancement of the quantum yield was observed in all of the C₃-C₄ intermediate species, ranging from 21% in F. ramosissima to 43% in F. pubescens. In all intermediates the quantum yields in 2% O₂ were intermediate in value to the C₃ and C₄ species, indicating a co-function of the C₃ and C₄ cycles in CO₂ assimilation. The low quantum-yield values for F. pubescens and F. floridana in 21% O₂ presumably reflect an ineffcient transfer of carbon from the C₄ to the C₃ cycle. The response of the quantum yield to four increasing O₂ concentrations (2–35%) showed lower levels of O₂ inhibition in the C₃-C₄ intermediate F. ramosissima, relative to the C₃ species. This indicates that the co-function of the C₃ and C₄ cycles in this intermediate species leads to an increased CO₂ concentration at the site of ribulose-1,5-bisphosphate carboxylase/oxygenase and a concomitant decrease in the competitive inhibition by O₂.Abbreviations PEP phosphoenolpyruvate - PGA 3-phosphoglycerate - RuBP ribulose-1,5-bisphosphate     

Human C4 haplotypes with duplicated C4A or C4B

In the course of study of families for the sixth chromosome markers HLA-A, C, B, D/DR, BF, and C2, the two loci for C4, C4A, and C4B, and glyoxalase I, we encountered five examples of probable duplication of one or the other of the two loci for C4. In one of these, both parents and one sib expressed two different structural genes for C4B, one sib expressed one, and one sib expressed none, suggesting that two C4B alleles were carried on a single haplotype: HLA-A2, B7, DR3, BFS1, C2C, C4A2, C4B1, C4B2, GLO1. In a second case, two siblings inherited C4B*1 and C4B*2 from one parent and C4B*Q0 from the other. This duplication appeared on the chromosome as HLA-AW33, B14, DR1, BFS, C2C, C4A2, C4B1, C4B2, GLO2. In a third, very large family with 3 generations, a duplication of the C4B locus occurred which was followed in 2 generations. In one individual, there were three C4B alleles and two C4A alleles. One of the C4B alleles had a hemolytically active product with electrophoretic mobility near C4B2 and was designated C4B*22. It segregated with C4B1 in the family studied. The complete haplotype was HLA-A11, CW1, BW56, DR5, BFS, C2C, C4A3, C4B22, C4B1, GLO2. In another family with 12 siblings, one parent and eight children expressed two C4A alleles on the haplotype HLA-AW30, BW38, DR1, BFF, C2C, C4A3, C4A2, C4BQ0, GLO1.(ABSTRACT TRUNCATED AT 250 WORDS)