日本松干蚧的重要天敌——隐斑瓢虫的初步研究

隐斑瓢虫是近年来在杭州地区发现的日本松干蚧的一种重要捕食性天敌。该虫在杭州一年发生四代,其年发生规律基本上和日本松干蚧的生活周期相吻合,而且能在松林中形成比较稳定的群落。根据测定,隐斑瓢虫对日本松干蚧各虫态的捕食能力较强,一头成虫的日平均捕食量为:显露若虫13.33头,雌成虫4.27头,卵囊3.67个(每个卵囊内平均有卵265.5粒),雄蛹28.27只;一头幼虫全期(或2—4龄和3—4龄)分别能捕食显露若虫39.20—105.56头,雌成虫40.80—47.79头,卵囊39.38—41.79个,雄蛹220.50只。它在引进辽宁省沈阳和旅大地区后,不仅仍能正常的捕食日本松干蚧(显露若虫),其成虫和幼虫喂以各种蚜虫均能正常生殖和发育,并且一年可以繁殖三代:冬季,只要在0℃以上的温度条件下,给予少量的糖水等作补充营养,亦能安全的越冬。据此,作者认为隐斑瓢虫在浙江杭州和辽宁,均具有作为控制日本松干蚧的发生来加以饲养繁殖与利用的价值。     

苏芸金杆菌感染粘虫后中肠组织学病变的研究

本文描述了Bacillus thuringiensis HD-1纯晶体感染粘虫Mythimna separata 5龄初幼虫后,其中肠肠壁细胞的超微结构变化.电镜观察表明:首先线粒体,发生病变,随后,细胞顶部肿胀、胞质电子密度下降,顶部胞质之下的各种细胞器均受损伤.随着病变加重,柱状细胞基膜内褶及杯状细胞质突起,这两个富含线粒体的区域发生病变最为明显.最终,肠壁细胞解体从基膜脱落.     

Ca~(2 )对叶绿体中超氧物自由基产生以及由ACC形成乙烯的影响

高浓度Ca~(2 )(0.1 mol/L)使叶绿体产生O_2~ 的能力下降,旋转相关时间(τ_c)增大34.3％,即膜的流动性降低,并抑制ACC形成乙烯;衰老时细胞内的Ca~(2 )作用却与此相反;O_2~ 的生成与乙烯的产量成正相关(r=0.941)。EGTA,吩噻嗪和W_7等加入到叶绿体反应体系中,可使O_2~ 的产量下降,ACC形成乙烯减少;相反,亚油酸作为Ca~(2 )载体,却使之明显升高,但亚油酸本身产生乙烯的量比ACC少得多。因此推测:高浓度Ca~(2 )可能影响叶绿体膜的状态,从而影响EFE的构象或者减少O_2~ 的生成,抑制ACC的转化,衰老时细胞内的Ca~(2 )可启动钙信使系统,使O_2~ 的产量升高,而其中膜脂过氧化是衰老的中心环节,因此O_2~ 的升高可能是诱发衰老启动的重要因素。     

粪产碱菌(Alcaligenes faecalix)基因文库的构建和nifH基因同源顺序的克隆

采用λ噬菌体置换型载体EMBL4,构建了Alcaligenes faecalis A-15 H1菌株总DNA的基因文库。用Sau3AⅠ限制酶完成部分酶切,取13—20kb大小的片段进行克隆。载体DNA经BamHⅠ和SaiⅠ完全双酶切,左右臂“退火”形成左右臂载体分子后再与外源片段连接。左右臂载体分子与外源片段按照1:1的分子比进行体外连接。用E.coli BHB2688和E.coli BHB2690制备的包装抽提物进行体外包装,所得基因文库效价测定为1.2×10~6 pfu,远远超过理论上所需的库容量。以nif H基因作为探针,经3轮噬菌斑原位杂交,从基因文库中筛选出含有其同源顺序的克隆,并得到了梯度点杂交的验证。对所得重组噬菌体克隆之一进行Southern转移杂交,结果证实,其3.5kb的EcoRⅠ酶切片段为nif H阳性杂交条带。将其克隆到质粒pUC19 DNA上后,转入受体菌JM101中。再次经Southern转移杂交,证明所得重组质粒克隆(pAFH)含有粪产碱菌中的与nifH基因有同源顺序的片段。     

Cis-trans isomerization of an angiotensin I-converting enzyme inhibitor. An enzyme kinetic and nuclear magnetic resonance study

The angiotensin I-converting enzyme (peptidyl-dipeptide hydrolase, EC 3.4.15.1) inhibitor, ramiprilat (2-[N-[(S)-1-ethoxycarbonyl-3-phenylpropyl]-L-Ala]-(1S,3S,5S)-2- azabicyclo[3.3.0]octane-3-carboxylic acid), is shown to exist in tow conformational isomers, cis and trans, which interconvert around the amide bond. The two conformers were separated by reversed-phase high-performance liquid chromatography. The conformers were identified by nuclear Overhauser effect measurements. From line shape analysis the isomerization rate constants were determined to be kcis----trans = 15 s-1 and ktrans----cis = 5 s-1 at 368 K in [2H]phosphate buffer (p2H 7.5). By enzyme kinetic studies using 3-(2-furylacryloyl)-L-Phe-Gly-Gly as substrate, the trans conformer was found to be the most potent enzyme inhibitor, whereas the cis conformer had a very low inhibitory effect. A new inhibition mechanism is presented for this type of slow, tight-binding inhibitors that contain an amide bond. This mechanism involves an equilibrium between the two conformers and the enzyme-bound inhibitor complex.     

db—cAMP对转化细胞钙调素基因表达与细胞骨架的影响

We have demonstrated that the distribution of microtubules (MT), microfilaments (MF) and fibronectin (FN) were diminished, while the gene expression of the calmodulin and c-fos enhanced in the transformed C3 H10 T1/2 cells. After treatment with 1 mM db-cAMP for 1 hr. and 2 hrs., there was an early and rapidly reduced in gene expression of calmodulin and c-fos respectively. After db-cAMP treatment for 4-5 days, the number of Capping cells of ConA binding decreased significantly and the cell surface microvilli decreased also. The growth of treated cells was inhibited markedly. By using 4F1 cDNA probe, which is preferentially expressed in G1 phase, we have found that the db-cAMP treated cells were accumulated at G1 phase. Of particular interest is the fact that the distribution of microtubules, microfilaments and fibronectin were recovered after treatment with 1 mM db-cAMP for 6 days. It is suggested that the inhibition of proliferation, alteration of phenotype and recovery of cytoskeleton in transformed cells after treatment with db-cAMP are related to the inhibition of gene expression of calmodulin.     

中国狭长蝽属初记(半翅目:长蝽科:杆长蝽亚科)

狭长蝽属(Dimorphopterus Stal)为杆长蝽亚科(Blissinae)中较大的一属。身体常成两侧平行的小杆状,多数尚较粗壮,亦有甚狭长者,体黑,被平伏或半直立毛,翅革片白色而有深色斑,常出现短翅型个体。多生活于禾本科植物上,北方地区为害高粱的“高粱长蝽”即属此类。 本属的概念和范围几经变动:Stal 1872年建立此属时,用身体较狭,触角短于头、胸     

Two contiguous thrombin fragments of human somatotropin form a functionally active recombinant, but the two homologous fragments from sheep hormone do not

Two thrombin fragments of reduced-carbamidomethylated human somatotropin representing the full primary structure of the native hormone (residues 1-134 and 135-191) have been found to form a recombinant molecule with properties similar to those of reduced-carbamidomethylated human somatotropin as shown by circular dichroism spectroscopy, two receptor-binding assays, and radioimmunoassay. In contrast, the homologous thrombin fragments of reduced-carbamidomethylated sheep hormone (residues 1-133 and 134-191) do not undergo recombination. Furthermore, neither the reduced-alkylated nor the reduced and nonalkylated C-terminal thrombin fragment of sheep hormone is able to interact with the reduced-carbamidomethylated N-terminal thrombin fragment of human hormone, under conditions which favor the recombination of the two human somatotropin fragments.     

Purification and properties of malate dehydrogenase from Pseudomonas testosteroni.

Nicotinamide adenine dinucleotide-linked malate dehydrogenase has been purified from Pseudomonas testosteroni (ATCC 11996). The purification represents over 450-fold increase in specific activity. The amino acid composition of the enzyme was determined and found to be quite different from the composition of the malate dehydrogenases from animal sources as well as from Escherichia coli. Despite this difference, however, the data show that the enzymatic properties of the purified enzyme are remarkably similar to those of other malate dehydrogenases that have been previously studied. The Pseudomonas enzyme has a molecular weight of 74,000 and consists of two subunits of identical size. In addition to L-malate, the enzyme slowly oxidizes other four-carbon dicarboylates having an alpha-hydroxyl group of S configuration such as meso- and (-) tartrate. Rate-determining steps, which differ from that of the reaction involving L-malate, are discussed for the reaction involving these alternative substrates. Oxidation of hydroxymalonate, a process previously undetected with other malate dehydrogenases, is demonstrated fluorometrically. Hydroxymalonate and D-malate strongly enhance the fluorescence of the reduced nicotinamide adenine dinucleotide bound to the enzyme. The enzyme is A-stereospecific with respect to the coenzyme. Malate dehydrogenase is present in a single form in the Pseudomonas. The susceptibility of the enzyme to activation or inhibition by its substrates-particularly the favoring of the oxidation of malate at elevated concentrations-strongly resembles the properties of the mitochondrial enzymes. The present study reveals that whereas profound variations in chemical composition have occurred between the prokaryotic and eukaryotic enzymes, the physical and catalytic properties of malate dehydrogenase, unlike lactate dehydrogenase, are well conserved during the evolutionary process.