色氨酸阻遏物与其操纵基因复合物的圆二色性研究

用圆二色性谱来确定色氨酸阻遏物与其操纵基因复合物在溶液中的构象变化。色氨酸阻遏物的圆二色性图谱表明它是一种富含α螺旋的蛋白质,通过比较加入Ｌ－Ｔｒｐ前和后的圆二色性谱,发现活性的与非活性的色酸阻遏物二级结构变化很小,ｔｒｐ Ｐ／Ｏ的圆二色性谱与它的单健、双链理论计算曲线对比,可近拟推测操纵基因在溶液中的存在状态。用色氨酸阻遏物对ｔｒｐ Ｐ／Ｏ进行确定,可以从中找出蛋白质与核酸结合的平衡点。从平衡时     

棉纤维发育过程中细胞壁超微结构变化的研究

应用X射线衍射法研究了棉纤维发育过程中细胞壁超微结构变化的动态规律.其结果是:次生壁S_2层的平均微纤丝螺旋角随花后生长天数的增加而逐渐变小:纤维素微晶粒间的取向度逐渐变大;花后5—14天内,结晶度缓慢增加,14—17天内陡然增加,17天后缓慢趋向最大值.     

不同配体与同一膜受体结合的初步探讨

研究了伴刀豆球蛋白A(ConA)和层粘连蛋白(LN)与巨噬细胞膜受体竞争结合,初步推测两个配体与同一膜受体结合的可能性.结果表明,LN可以竞争抑制FTTC-ConA与巨噬细胞膜受体的结合,说明ConA和LN两种配体各自的巨噬细胞膜受体中有部分可能是共同的,而加入ConA反而增加巨噬细胞膜上结合的FITC-LN量,这可能是因为ConA和LN的分子特性导致的.     

细胞分裂素在离体蒜苔内的运转

离体蒜苔饲喂带~3H 标记的6-苄基腺嘌呤(BA)后在暗中25℃下放置,分别在第3、5、10、15、20天取样,进行放射性物质的分布分析。结果表明:(1)BA 能沿着苔茎大量、长距离地上运,并在顶端的珠蒜中积累;(2)BA 的这种运转具有很强的向顶极性;(3)这种运转是一个平缓而稳定的过程,珠蒜中 BA 的积累与时间成较好的线性关系;(4)顶端的珠蒜对 BA 的上运是必不可少的。根据以上结果,本文对蒜苔内 BA 的运转机理及意义进行了讨论。     

变黄黑文衣,中国黑文衣属地衣一新记录种

通过对文字衣科黑文衣属形态学、解剖学、化学与分子生物学的研究,发现中国新记录种1种,即变黄黑文衣(Phaeographis flavescens Dal-Forno&Eliasaro),该种主要特征为地衣体壳状,表面浅黄绿色,无光泽,光滑;子囊盘弯曲,多分支,聚生于假子座中;盘缘黑色,相邻线盘之间有小缝隙,盘面较平坦,黑色,覆有白色粉霜;子囊层无色透明,侧丝顶端分支;子囊含8个子囊孢子;子囊孢子褐色,横隔透镜型,(4～)6胞室,大小19～25.5μm×6～7μm,I+紫红色。该种分布于云南和福建,该研究丰富了对中国黑文衣属物种组成与分布的认知。     

High-Resolution Performance of Polycaprolactone Functionalized with Guanidinium Ionic Liquid for Gas Chromatography

This work firstly reported a new polycaprolactone based material functionalized with guanidinium ionic liquid (PCL-GIL) as the stationary phase with high resolution performance for capillary gas chromatography (GC). It is composed of polycaprolactone (PCL) and guanidinium ionic liquid (GIL) with amphiphilic conformation. The PCL-GIL capillary column coated by static method exhibited high column efficiency of 3942 plates/m and moderate polarity. As a result, the PCL-GIL column exhibited high-resolution capability. For a mixture of 27 analytes with a wide ranging polarity and outperformed the PCL-2OH and HP-35 columns, showing its advantageous separation capability for analytes of diverse types. Moreover, the PCL-GIL column showed high resolving capability for various positional isomers and cis-/trans-isomers, including alkylbenzenes, chlorobenzenes, naphthalenes, bromonitrobenzenes, chloronitrobenzenes, benzaldehydes, phenols, alcohols, respectively. In a word, PCL derivatized by GIL units as a new type of stationary phase has a promising future in GC separations.     

A short-chain carbonyl reductase mutant is an efficient catalyst in the production of (R)-1,3-butanediol

R-1,3-butanediol (R-1,3-BDO) is an important chiral intermediate of penem and carbapenem synthesis. Among the different synthesis methods to obtain pure enantiomer R-1,3-BDO, oxidation–reduction cascades catalysed by enzymes are promising strategies for its production. Dehydrogenases have been used for the reduction step, but the enantio-selectivity is not high enough for further organic synthesis efforts. Here, a short-chain carbonyl reductase (LnRCR) was evaluated for the reduction step and developed via protein engineering. After docking result analysis with the substrate 4-hydroxy-2-butanone (4H2B), residues were selected for virtual mutagenesis, their substrate-binding energies were compared, and four sites were selected for saturation mutagenesis. High-throughput screening helped identify a Ser154Lys mutant which increased the catalytic efficiency by 115% compared to the parent enzyme. Computer-aided simulations indicated that after single residue replacement, movements in two flexible areas (VTDPAF and SVGFANK) facilitated the volumetric compression of the 4H2B-binding pocket. The number of hydrogen bonds between the stabilized 4H2B-binding pocket of the mutant enzyme and substrate was higher (from four to six) than the wild-type enzyme, while the substrate-binding energy was decreased (from −17.0 kJ/mol to −29.1 kJ/mol). Consequently, the catalytic efficiency increased by approximately 115% and enantio-selectivity increased from 95% to 99%. Our findings indicate that compact and stable substrate-binding pockets are critical for enzyme catalysis. Lastly, the utilization of a microbe expressing the Ser154Lys mutant enzyme was proven to be a robust process to conduct the oxidation–reduction cascade at larger scales.     

REGENERATION AND SEXUAL DIFFERENTIATION OF GRIFFITHSIA JAPONICA (CERAMIACEAE,RHODOPHYTA) THROUGH SOMATIC CELL FUSION1

Hybrid cells were obtained from somatic cell fusion among male, female, and tetrasporangial plants in Griffithsia japonica Okamura by a wound-healing process. Isolated fusion cells regenerated new mature plants with mixed reproductive structures. The plants regenerated from hybrid cells between male and female plants developed into 1) spermatangiate, 2) carpogonial, 3) bisexual with spermatangia and carpogonial branches, 4) mixed-phase with spermatangia and tetrasporangia, or 5) bisexual/mixed-phase plants with spermatangia, carpogonial branches, and tetrasporangia. About 70% of the plants regenerated from hybrid cells between male and female plants produced tetrasporangia that were always formed with spermatangia on a single cell. Some of those tetrasporangia released tetraspores, six of which gave rise to mature plants. The plants regenerated from hybrid cells between male and tetrasporangial plants developed into spermatangiate, tetrasporangiate, or mixed-phase plants with spermatangia and tetrasporangia. The plants regenerated from hybrid cells between female and tetrasporangial plants developed into carpogonial, tetrasporangiate, or mixed-phase plants with carpogonial branches and tetrasporangia. All types of reproductive structures we re functional.     

Crystal structure of Streptomyces diastaticus No. 7 strain M1033 xylose isomerase

The crystal structures of Streptomyces diastaticus No. 7 strain M1033 xylose isomerase (SDXyI) have been analysed and refined at 0.19nm. The crystal space group is I222, with unit cell dimensions of a=9.884 ran, b=9.393nm and c=8.798nm. Based on the coordinates of the Streptomyces rubiginosus xylose isomerase (SRXyI), the initial model of SDXyl was built up by the dose packing analysing and R-factor searching and refined by PROLSQ to a final R-factor of 0.177 with the rms deviations of bond lengths and bond angles of 0.001 9nm and 2.1°, respectively. No significant global conformation change existed between SRXyI and SDXyI except the local conformation in the active site.