大鼠心肌线粒体肌酶激酶肌模型亚基的克隆及其鉴定

根据以发表的大鼠心肌线粒体肌酸激酶肌模型亚基基因（ｓＭｉＭｉ－ＣＫ）的ｃＤＮＡ序列,设计并人工合成一对特异性引物,以大鼠心肌总ＲＮＡ为模板,反转录聚合酶链反应（ＲＴ－ＰＣＲ）扩增出一段编码大鼠心肌ｓＭｉＭｉ－ＣＫ的ＤＮＡ片段（１．３３ｋｂ）,将该片段克隆到载休ｐＵＣ１９上并进行初步鉴定,然后进行测序分析,结果与国外以报道的序列完全一致,证明已得到ｓＭｉＭｉ－ＣＫ基因,为今后ｓＭｉＭｉ－ＣＫ基因的表     

朝鲜淫羊藿的化学成分（Ⅱ）

从朝鲜淫羊藿的地上部分分离到七个成分（Ⅰ、Ⅱ、Ⅲ、Ⅳ、Ⅴ、Ⅵ、Ⅶ）。经ＵＶ,ＩＲ,＾１Ｈ－ＮＭＲ,＾１３Ｃ－ＮＭＲ,ＭＳ及化学方法鉴定了它们的结构,分别是ｉｃａｒｉｔｉｎ－３－Ｏ－ａ－Ｌ－ｒｈａｍｎｏｐｙｒａｎｏｓｉｄｅ（Ⅰ）,ｓａｇｉｔｔａｔｏｓｉｄｅ Ａ（Ⅱ）,ｓａｇｉｔｔａｔｏｓｉｄｅ Ｂ（Ⅲ）,３,５,７－ｔｒｉｈｙｄｒｏｘｙｌ－４＾１－ｍｅｔｈｏｘｙ１－８－ｐｒｅｎｙ１－ｆｌａｖｏｎｅ－     

6－Dimethylaminopurine（6－DMAP） Spontaneously Induces Interphase Transition Of Metaphase Mouse Oocytes

６－Ｄｉｍｅｔｈｙｌａｍｉｎｏｐｕｒｉｎｅ（６－ＤＭＡＰ）ＳｐｏｎｔａｎｅｏｕｓｌｙＩｎｄｕｃｅｓＩｎｔｅｒｐｈａｓｅＴｒａｎｓｉｔｉｏｎＯｆＭｅｔａｐｈａｓｅＭｏｕｓｅＯｏｃｙｔｅｓ￥ＳＵＮＱｉｎｇ－ｙｕａｎ（孙青原）;ＧＡＯＳｈａｏ－ｒｏｎｇ（高...     

人端粒酶RNA基因的克隆与鉴定

以人血基因组ＤＮＡ为模板,合成两段２０个寡聚核苷酸为引物,经过ＰＣＲ扩增,得到４８０ｂｐ的片段,克隆到ｐＭＤ１８－Ｔ载体中,经电泳、酶切、ＰＣＲ鉴定后测定序列。序列分析表明氙克隆的人端粒酶ＲＮＡ（ｈｕｍａｎ ｔｅｌｏｍｅａｓｅ ＲＮＡ,ｈＴＲ）基因含有４８０ｂｐ,包括约４５０ｂｐ的编码模板区主序列和约３０ｂｐ的上游调控区序列,其中模板区的１１个核苷酸（５’－ＣＵＡＡＣＣＣＵＡＡＣ－３’）合成端粒亚     

大火草要部的化学成分

大火草（Ａｎｅｍｏｎｅｔｏｍｅｔｏｓ（Ｍａｘｉｍ）Ｐｅｉ）根状茎提取物的乙酸乙酯部分对粘虫（ＬｅｕｃａｎｉａｓｅｐａｒａｔａＷａｌｋｅｒ）有较好的非选择性拒食活性。从该部分分离得到１１个化合物,通过ＮＭＲ、ＭＳ等波谱分析确定它们的结构分别为４,５－二甲氧基－７－甲基香豆素（１）、４－     

抗水稻矮缩病毒的反义核酶及复制酶部分序列的合成、克隆及其水稻表达载体的构建

采用反转录－聚合酶链式反应方法（ＲＴＰ－ＣＲ）,在人工合成的引物引导下,扩增出水稻矮缩病毒基因组第一片段（Ｓ１）全长序列及第五片段的部分序列（ＳＳⅢ）．将扩增的片段分别克隆到克隆载体ｐＧＥＭ７Ｚｆ（＋）及ｐＵＣ１９的ｓｍａｌ位点上,并进行了序列测定。在此基础上,利用ｐＣＲ引入的方法将核酶序列引入到Ｓ５Ⅲ片段反义链上以构成反义核酶基因Ｓ５ⅢＲ,将Ｓ１片段５＇端部分序列（Ｓ１－１）及Ｓ５ⅢＲ基因克隆到植物表达载体ｐＲＯＫⅡ上,构建成水稻转化载体ｐＲＯＫ－Ｓ１－１＇及ｐＲＯＫ－Ｓ５ⅢＲ。     

灯盏细辛中酚类化合物的化学研究

从灯盏细辛（Ｅｒｉｇｅｒｏｎ ｂｒｅｖｉｓｃａｐｕｓ（Ｖａｎ．）Ｈａｎｄ－Ｍａｚｚ）的乙酸乙酯部分首次分离得到５个二咖啡酰基的酚类化合物（１￣５）和９个其他类型化合物。其中ｅｒｉｇｏｓｔｅｒ Ａ（１）为一全新骨架的化合物。利用波谱方法（＾１Ｈ－ＮＭＲ,＾１３Ｃ－ＮＭＲ,２Ｄ－ＮＭＲ和ＦＡＢ－ＭＳ等）对这些化合物的结构进行了鉴定。     

Dynamic Changes of β Tubulin during the Resumption of Meiosis of Mouse Oocyte

ＤｙｎａｍｉｃＣｈａｎｇｅｓｏｆβＴｕｂｕｌｉｎｄｕｒｉｎｇｔｈｅＲｅｓｕｍｐｔｉｏｎｏｆＭｅｉｏｓｉｓｏｆＭｏｕｓｅＯｏｃｙｔｅＬＩＵＨｕｉ;（刘辉）ＣＨＥＮＤａ－ｙｕａｎ;（陈大元）（ＳｔａｔｅＫｅｙＬａｏｂｏｒａｔｏｒｙｏｆＲｅｐｒｏｄｕｃｔｉ...     

大鼠心肌线粒体肌酸激酶肌膜型亚基的克隆及其鉴定

根据以发表的大鼠心肌线粒体肌酸激酶肌膜型亚基基因（ｓＭｉＭｉＣＫ）的ｃＤＮＡ序列,设计并人工合成一对特异性引物,以大鼠心肌总ＲＮＡ为模板,反转录聚合酶链式反应（ＲＴＰＣＲ）扩增出一段编码大鼠心肌ｓＭｉＭｉＣＫ的ＤＮＡ片段（１．３３ｋｂ）,将该片段克隆到载体ｐＵＣ１９上并进行初步鉴定,然后进行测序分析,结果与国外以报道的序列完全一致,证明已得到ｓＭｉＭｉＣＫ基因,为今后ｓＭｉＭｉＣＫ基因的表达创造了良好的条件     

竹中花椒化学成分研究

从竹叶花椒（ＺａｎｔｈｏｘｙｌｕｍａｒｍａｔｕｎＤＣ．）树皮中分离１３种化合物,经波谱（ＵＶ,ＩＲ,ＮＭＲ,ＭＳ）分析及理化常数的对照,鉴定其其中的９种,它们是：β－白檀酮（β－ａｍｙｒｏｎｅ）（Ⅱ）β－香木脂醇（β－ａｍｙｒｉｎ（Ⅱ）,Ｌ细辛素（Ｌ－ａｓａｒｉｎｉｎ（Ⅳ）Ｌ－芝麻素（Ｌ－ｓｅｓａｍｉｎｉ（Ⅴ）,－ＤＬＤ－竹叶椒脂素（Ｌ－ｐｌａｎｉｎｉｎ（Ⅵ）β－胡萝卜甙（β－ｄａｕｃｏｓｔｅｒｏ     

Cloning and expression of Drosophila melanogaster UDP-GlcNAc:alpha-3-D-mannoside beta1,2-N-acetylglucosaminyltransferase I

A TBLASTN search of the Drosophila melanogaster expressed sequence tag (EST) database with the amino acid sequence of human UDP-N-acetylglucosamine:alpha-3-D-mannoside beta-1,2-N-acetylglucosaminyltransferase I (GnT I, EC 2.4.1.101) as probe yielded a clone (GM01211) with 56% identity over 36 carboxy-terminal amino acids. A 550 base pair (bp) probe derived from the EST clone was used to screen a Drosophila cDNA library in lambda-ZAP II and two cDNAs lacking a start ATG codon were obtained. 5'-Rapid amplification of cDNA ends (5'-RACE) yielded a 2828 bp cDNA containing a full-length 1368 bp open reading frame encoding a 456 amino acid protein with putative N-terminal cytoplasmic (5 residues) and hydrophobic transmembrane (20 residues) domains. The protein showed 52% amino acid sequence identity to human GnT I. This cDNA, truncated to remove the N-terminal hydrophobic domain, was expressed in the baculovirus/Sf9 system as a secreted protein containing an N-terminal (His)6 tag. Protein purified by adsorption to and elution from nickel beads converted Man alpha1-6(Man alpha1-3)Man beta-octyl (M3-octyl) to Man alpha1-6(GlcNAc beta1-2Man alpha1-3)Man beta-octyl. The Km values (0.7 and 0.03 mM for M3-octyl and UDP-GlcNAc respectively), temperature optimum (37 degrees C), pH optimum (pH 5 to 6) and divalent cation requirements (Mn > Fe, Mg, Ni > Ba, Ca, Cd, Cu) were similar to mammalian GnT I. TBLASTN searches of the Berkeley Drosophila Genome Project database with the Drosophila GnT I cDNA sequence as probe allowed localization of the gene to chromosomal region 2R; 57A9. Comparison of the cDNA and genomic DNA sequences allowed the assignment of seven exons and six introns; all introns showed GT-AG splice site consensus sequences. This is the first insect GnT I gene to be cloned and expressed.     

Isolation and mapping of a putative b subunit of human ATP synthase (ATP-BL) from human leukocytes.

From a human-leukocyte cDNA library, we cloned cDNA encoding a novel protein, which has a significant homology with the b subunit of ATP synthase (proton-transporting ATPase, F1F0-ATPase; EC3.6.1.34) derived from Anabaena sp. strain PCC 7120. The cDNA has an open reading frame of 1314 nucleotides corresponding to 438 amino acids. The coding sequence was 37.9% identical over 57 amino acid with b subunit of ATP synthase. The 34-amino-acid region of the predicted peptide sequence displays a coiled-coil motif that could form a complex with some other protein(s). We designated this novel gene as ATP-BL because of its homology to the b subunit of ATP synthase. The ATP-BL locus was mapped by fluorescence in situ hybridization (FISH) and radiation hybrid mapping to the q24 region of chromosome 16.     

Structural analysis of the sequence coding for an inducible 26-kDa protein in human fibroblasts

When human fibroblast cells were stimulated with poly(I) X poly(C) in the presence of cycloheximide for the production of interferon-beta (IFN-beta), a 26-kDa protein could be immunoprecipitated by antiserum raised against partially purified human IFN-beta [Content, J., De Wit, L., Pierard, D., Derynck, R., De Clercq, E. & Fiers, W. (1982) Proc. Natl Acad. Sci. USA 79, 2768-2772]. In our hands this 26-kDa protein showed no antiviral activity. Other investigators have, however, reported the presence in the same conditions of a second type of IFN, a so-called beta 2 species [Weissenbach, J., Chernajovsky, Y., Zeevi, M., Shulman, L., Soreq, H., Nir, U., Wallach, D., Perricaudet, M., Tiollais, P. & Revel, M. (1980) Proc. Natl Acad. Sci. USA 77, 7152-7156] of which the mRNA structure and protein characteristics strongly suggests identity with the 26-kDa product. In this paper we describe the nucleotide sequence of the 26-kDa cDNA and part of the corresponding genomic clone. The cDNA clones were isolated from a library made with mRNA from induced human fibroblasts. As, however, the information thus obtained was still incomplete, genomic clones were isolated from a total human DNA library. In this way, the entire region coding for the 26-kDa protein was established, as well as the neighbouring sequences including the inducible promoter area. From the deduced polypeptide sequence a number of characteristics of the 26-kDa protein can be explained. It turns out that the 26-kDa protein gene and the so-called 'IFN-beta 2' gene are identical. However, extensive homology searches indicate that the 26-kDa protein does not show statistically significant sequence homology with any known interferon species. Hence, the question of whether the 26-kDa product represents a novel IFN species remains open.     

Isolation and mapping of rFUS6, a rice orthologue of Arabidopsis thaliana FUS6.

COP9 complex is one of the most important components that act in repressing photomorphogenesis in Arabidopsis thaliana. FUS6 has been identified as one of eight subunits of the COP9 complex in Arabidopsis. Using Arabidopsis Fus6 cDNA as a probe, we screened a rice root cDNA library and a rice genomic library. A 1730-bp cDNA was obtained, which has an open reading frame corresponding to 441-amino-acid. This 441 amino acids putative protein has 67% identity with Arabidopsis COP11/FUS6 (AtFUS6) and 40% identity with human GPS1, an AtFUS6 orthologue. So we designated this novel gene as rFUS6. The 6.2-kb genomic sequence of rFUS6 was also obtained. Sequence comparison showed that the rFUS6 gene had six exons and five introns. Sequence inspection of the 5'-flanking region revealed the presence of some potential light-regulated cis-elements such as a G-box, GT-1 binding sites, and a TGACG motif. Southern hybridization with rice total DNA showed that rFUS6 was perhaps a single copy gene. The rFUS6 locus was mapped by hybridization with a rice BAC library membrane and the results showed that rFUS6 had a locus at 16.3 cM of chromosome 1.     

肺形侧耳变温结实相关基因Ppcsl-1的克隆及功能预测

CSL（CBF1/RBP-Jκ/suppressor of hairless/LAG-1）转录因子家族在真菌发育和细胞分化过程中扮演重要角色。前期研究已构建了肺形侧耳变温结实相关消减杂交文库,并从中筛选到一个代表csl基因部分序列的EST。通过TAIL PCR（thermal asymmetric interlaced PCR）技术克隆了该基因（Pleurotus pulmonarius csl-1,简写为 Ppcsl-1）,并利用RACE（rapid-amplification of cDNA ends）技术获得该基因的cDNA全长。Ppcsl-1 cDNA全长2 991bp,编码一个996个氨基酸组成的蛋白（命名为PpCSL-1）。进化分析显示在担子菌CSL中,PpCSL-1与糙皮侧耳Pleurotus ostreatus CSL（PoCSL）亲缘关系最近。荧光定量检测结果表明Ppcsl-1在菌丝经过5℃ 12h冷处理之后的表达量最高,表明其有可能被冷刺激诱导表达并在开启子实体形成的过程中起重要作用。     

Cloning of rat brain protein kinase C complementary DNA

Four peptides derived from rat brain protein kinase C were partially sequenced. Using synthetic oligonucleotides deduced from the amino acid sequences as probes, a clone of complementary DNA (cDNA) was isolated from a cDNA library prepared from the same tissue. The nucleotide sequence of this cDNA clone revealed the primary structure of the carboxyl-terminal region as having 224 amino acids, with significant sequence homology with cyclic AMP-dependent and cyclic GMP-dependent protein kinases.