西藏土壤中铜含是及分布

1　引　　言目前 ,西藏的生态环境基本保持原生状态 ,是至今地球上受人类活动影响和污染最少的地区之一 .所以 ,西藏是进行生态环境本底调查和表生地球化学研究最为理想的场所 .西藏的土壤中Ｃｕ含量数据 ,不但有助于进一步研究西藏高原表生环境中Ｃｕ的地球化学特征 ,而且还可以为这一地区环境监测与评价等提供基础信息和依据 ,也可以成为全国乃至全世界土壤生态环境背景的永久性参比资料 .2　材料与方法2 1　供试材料样品采自北起唐古拉山 ,南至亚东、樟木、吉隆、普兰 ,东从金沙江 ,西到班公错—除羌唐高原北部以外的西藏广大地区 ,共计…     

西藏土壤中铜含量及分布

Cu content in soils sampled from different sites in Tibet was analyzed.The results showed that the average Cu content of soils was 19.6mg穔g^-1,lower than the average content in China.The content of Cu was distributed in Tibet with a total of gradually decreasing from the southeast to the northwest,which was consistent with the direction of change in the zonal successions of soil in Tibet.The variation of the content of Cu in the soils developed from different soil parent materials in Tibet was very remarkable,and the content of Cu in the soil developed from shale was greatly higher than that in the soil developed from other soil parent material.     

Effect of ethanol on activity of the plasma-membrane ATPase in, and accumulation of glycine by, Saccharomyces cerevisiae

The pH optimum of the ATPase activity in plasma membranes from Saccharomyces cerevisiae NCYC 431 from 8 h cultures was around 6.5 and that in membranes from organisms from 16 h cultures near 6.0. The Km[ATP] of the enzyme was virtually unaffected by the age of the culture from which organisms were harvested, although the Vmax of the enzyme in membranes from organisms from 8 h cultures was higher than that for organisms from 16 h cultures. Ethanol non-competitively inhibited ATPase activity in membranes, although the inhibition constant for the enzyme from organisms from 8 h cultures was lower than that from organisms from 16 h cultures. Glycine accumulation by the general amino acid permease was non-competitively inhibited by ethanol. Inhibition constants were virtually the same for glycine uptake by deenergized organisms from 8 h and 16 h cultures, but under energized conditions the value was greater for organisms from 16 h rather than 8 h cultures. The data indicate that inhibition of plasma-membrane ATPase activity by ethanol could account, at least in part, for inhibition of glycine accumulation by ethanol.     

Colour remediation of pulp mill effluent using purified fungal cellobiose dehydrogenase: reaction optimisation and mechanism of degradation

Cellobiose dehydrogenase purified from two different fungal sources was assessed for its ability to remove and/or reduce colour from pulp mill bleach plant effluent. Cellobiose dehydrogenase purified from Phanerochaete chrysosporium was shown to prefer acidic conditions and was consequently used to treat the acid effluent stream discharged from a pulp mill bleach plant, while an analogous enzyme originating from Humicola insolens preferred alkaline conditions, and was applied to the effluent discharged from the caustic sewer of the bleach plant. Both enzyme preparations were able to remove colour from their respective effluent sources to a comparable extent. Up to 50% of the effluent colour was removed within 4 days when treated under optimised conditions. Furthermore, it was also shown that this enzymatic approach was effective at removing colour generated by both softwood and hardwood resources. Mechanistically, it was shown that colour was removed from all molecular weight fractions, and the higher molecular weight material (>300 kDa) was concurrently preferentially degraded. Cellobiose dehydrogenase treatment of effluent did not target phenolic, stilbene, or alpha-carbonyl structures, but did affect the quinone content. Further investigations using model compounds confirmed these results, and subsequently showed that only the para-quinones with low substitution were reduced with cellobiose dehydrogenase.     

The Prevalence of Listeria monocytogenes in the Environment of Dairy Farms

The prevalence of Listeria monocytogenes in the environment of dairy farms was surveyed from December 1993 to June 1994 in one city of Hokkaido. L. monocytogenes was isolated from 3 out of 5 farms investigated. Serovar 4b organism was isolated from the brain stem of a cow from one farm which was clinically diagnosed as having listeriosis. The same serovar of L. monocytogenes was also isolated from the rectal contents of a healthy cow, straw on the floor, straw in the barn, and silage scattered around the silo from the same farm. At another farm, with no reported cases of bovine listeriosis, serovar 1/2 organism was isolated from the same types of samples as the above mentioned farm except from straw on the floor. The difference in the isolation rates of the organism from straw on the floor between the two farms (22%: 5/23 vs 0%: 0/24) is considered to be caused by the different feeding methods of silage between the two farms.     

Crystallographic analysis of the thermal motion of the inclusion complex of cyclomaltoheptaose (beta-cyclodextrin) with hexamethylenetetramine

The crystal structure of the inclusion complex of cyclomaltoheptaose (beta-cyclodextrin) with hexamethylenetetramine was determined at temperatures of 123, 173, 223, and 293 K. The rigid-body motion of the host and guest molecules was evaluated by means of the TLS method that represents the molecular motion in terms of translation, libration, and screw motion. In increasing the temperature from 123 to 293 K, the amplitude of the rigid body vibration of the host molecule was increased from 1.0 to 1.3 degrees in the rotational motion and from 0.16 to 0.17 A in the translational motion. The cyclomaltoheptaose molecule has the flexibility in seven alpha-(1-->4)-linkages, and each glucose unit was in the rotational vibration around an axis through two glycosidic oxygen atoms. As a result, the rigid-body parameters of cyclomaltoheptaose were considered to be overestimated because of including the contribution from the local motion of glucose units. In contrast, for the guest molecule having no structural flexibility, the TLS analysis demonstrated that the atomic thermal vibration was mostly derived from the rigid body motion. The rotational amplitude of hexamethylenetetramine was changed from 5.2 to 6.6 degrees in increasing the temperature from 123 to 293 K, while the change of the translational amplitude was from 0.20 to 0.23 A. The translational motion of the guest molecule was hindered by the inside wall of the host cavity. The molecular motion was characterized by the rotational vibration around the axis through two nitrogen atoms that were involved in the hydrogen-bond formation.     

Biosynthesis of pyrethrin I in seedlings of Chrysanthemum cinerariaefolium

The biosynthetic pathway to natural pyrethrins in Chrysanthemum cinerariaefolium seedlings was studied using [1-13C]d-glucose as a precursor, with pyrethrin I isolated using HPLC from a leaf extract. The 13C NMR spectrum of pyrethrin I from the precursor-administered seedlings indicated that the acid moiety was biosynthesized from d-glucose via 2-C-methyl-d-erythritol 4-phosphate, whereas the alcohol moiety was possibly biosynthesized from linolenic acid.     

泰泽病原体基因组DNA提取方法的建立

目的　提取泰泽病原体基因组DNA ,为建立该菌基因组文库奠定基础。方法　使用密度梯度离心结合酶解消化方法、酶解消化方法、本研究建立方法即过滤盐析离心法 ,从感染肝脏组织纯化泰泽病原体 ,并比较三种方法纯化泰泽病原体效果 ;采用氯化苄法、试剂盒、酚法提取泰泽病原体基因组DNA ,并比较三种方法提取基因组DNA质量 ;鉴定酚法提取泰泽病原体基因组DNA特异性。结果　使用过滤盐析离心法从感染肝脏组织纯化泰泽病原体 ,采用酚法提取其基因组DNA ,所获得的基因组DNA特异性好、纯度高、DNA片段长度大于 5 0kb ,且均一性好 ,无降解。结论　本研究首次成功提取泰泽病原体基因组DNA ,可用于多种分子生物学实验     

Use of collagenase from the hepatopancreas of the Kamchatka crab for isolating and culturing endothelial cells of the large vessels in man

The application of hepatopancreas collagenase from crab Paralithodes camtschatica for the isolation and cultivation of the endothelial cells was studied in human umbilical vein endothelium. The comparison of the enzyme from crab hepatopancreas with collagenase from Clostridium histoliticum has shown that the number of viable cells isolated from human umbilical vein by the crab enzyme was lower than in the case of microbial collagenase. However, this difference was not significant for subsequent cultivation of cells. Harvesting of the endothelial cells from the substrate during cultivation was more effective in the case when collagenase from crab hepatopancreas was used. It was shown that crab collagenase, in contrast with microbiological collagenase, was not a metal-dependent enzyme.     

Isolation of protoplasts from somatic embryos of carrot

Protoplasts were isolated enzymatically from synchronously induced globular somatic embryos from a carrot suspension culture. Among the macerating enzymes tested, Driselase was the most effective for release of protoplasts from embryos. A higher medium osmolarity was required for the isolation of protoplasts from embryos than from undifferentiated cells. Protoplasts from embryos were smaller than protoplasts from undifferentiated cells. On step gradients of Ficoll, protoplasts from embryos gave one major band. Protoplasts from undifferentiated cells gave two major bands, one lighter and the other heavier than the protoplasts from embryos.     

酿酒酵母超氧物歧化酶(SOD)基因的克隆和表达

通过PCR扩增技术从酿酒酵母中得到了Cu,zn—SOD的结构基因,此基因被亚克隆到大肠杆菌质粒载体pT7—7．得到重组质粒pT7－7：SOD。利用EcoRI和Pstl酶切pT7-7::SOD质粒．经琼脂糖凝腔电泳,DEAE-滤膜回收Cu。zn—SOD结构基因片段,将其亚克隆到M13中．并转化大肠杆菌,得到了重组质粒M13-::t SOD,酶切和纯化后的SOD基因,定向克隆到酵母质粒载体pHz－8的smal和EcoRI位点上,构建成重组质粒pHZ－8－l。经转化酵母受体菌ZH-l和DP—l后得到了转化子．来自于ZH—l的转化子在非选择性条件下培养40世代后仍有95％以上细胞保留重组质粒。而来自于DP-1的转化子很不稳定。经蛋白提取、聚丙烯酰胺凝胶电泳和酶活性测定结果表明,来自于zH－1转化子中SOD的表达量约为细胞可溶性蛋白的15％．并具有生物活性。     

Parasitism of cowpea by Striga gesnerioides: variation in virulence and discovery of a new source of host resistance

In glasshouse experiments in the United Kingdom, Striga gesnerioides-resistant cowpea varieties, Suvita-2 and 58–57, were assessed alongside a susceptible variety for their responses to seventeen samples of S. gesnerioides from four West African countries. The susceptible variety was attacked by all samples, while Suvita-2 was resistant to samples from Burkina Faso and Mali, and 58–57 was resistant only to samples from Burkina Faso.
At least three physiological groups of the parasite can be distinguished: samples from Burkina Faso attacking the smallest range of cowpea varieties; those from Mali being intermediate; those from Niger and Nigeria attacking all the cowpea varieties. A sample from Cameroon behaved slightly differently and may represent a fourth type.
A cowpea line from Botswana, B.301, selected for its field resistance to Alectra vogelii proved resistant to all Striga populations to which it was exposed, including those from Niger and Cameroon.     

广东古兜山自然保护区森林生态系统服务价值评估

森林生态系统对维持自然生态系统格局、功能和过程具有特殊的生态意义。该文以广东省古兜山自然保护区为例,探讨了自然保护区森林生态系统服务功能的价值。采用市场价值法、影子工程法、替代花费法等对古兜山自然保护区森林生态系统服务功能价值进行评估,得出古兜山自然保护区每年森林生态系统服务功能总价值为57887615元。其中生产功能价值为6937700元,每年森林景观与游憩的平均价值为4050000元,森林生态系统改善大气环境的年总价值约32212700元,涵养水源与净化水质的年总价值为5809000元,森林保育土壤的年总价值为8878215元。该研究的目的在于以数值来显示自然保护区森林生态系统所提供的生态服务功能价值是巨大的,从而加深全社会对生态服务价值的认识,加强对森林生态系统服务功能的管理与保护。     

太湖一级保护区非点源磷污染的定量化研究

采用田间实验与实地调查相结合的方法,研究了太湖一级保护区武进市雪堰镇水稻季节各种类型非点源磷污染的负荷分配情况。结果表明,雪堰镇各种类型农业非点源污染中,农田磷排放总量为1313kg,占排放总量的56．2％;农村居民磷排放总量为442kg,占排放总量的18．9％;城镇居民磷排放总量为518kg．占排放总量的22．2％;养殖业磷排放总量为62kg,占排放总量的2．7％．在当前的非点源磷污染治理中,除采取有力措施控制农田养分外,对于城镇和农村居民生活污水和人粪尿的排放也应引起重视。     

Biotransformation of D-methionine into L-methionine in the cascade of four enzymes

D-Methionine was converted to L-methionine in a reaction system where four enzymes were used. D-amino acid oxidase (D-AAO) from Arthrobacter protophormiae was used for the complete conversion of D-methionine to 2-oxo-4-methylthiobutyric acid. Catalase was added to prevent 2-oxo-4-methylthiobutyric acid decarboxylation. In the second reaction step, L-phenylalanine dehydrogenase (L-PheDH) from Rhodococcus sp. was used to convert 2- oxo-4-methylthiobutyric acid to L-methionine, and formate dehydrogenase (FDH) from Candida boidinii was added for NADH regeneration. Enzyme kinetics of all enzymes was analyzed in detail. Mathematical models for separate reactions steps, as well as for the complete system were developed and validated in the batch reactor experiments. Complete conversion of D-methionine to L-methionine was achieved. Considering that both enzymes act on different substrates, such a system could be easily employed for the synthesis of other amino acids from D-isomer, as well as from the racemate of a certain amino acid (DL-amino acid).     

Noncryogenic Preservation of Mammalian Tissues for DNA Extraction: An Assessment of Storage Methods

Reliable field methods for the storage of tissues to be used for DNA extraction and amplification are critical to many studies employing molecular techniques. Protection from DNA degradation was compared among three commonly used methods of noncryogenic storage of tissues over a time scale of 2 years. All three methods prevented DNA degradation during storage for at least 6 months. DMSO (dimethyl sulfoxide)-salt solution provided the best protection from DNA degradation of tissues stored for up to 2 years. High molecular weight DNA was recovered from lysis buffer in which tissue was stored for 2 years, however, moderate amounts of degraded DNA was also present. High molecular weight DNA was recovered from tissues stored in ethanol for 2 years, however, the yield was relatively small compared to the other two noncryogenic storage techniques. Much of the DNA degradation in ethanol preserved tissues appeared to occur during the extraction procedure and can be reduced by soaking the tissue in lysis buffer for a few hours prior to beginning the extraction. The yield of PCR products was greatest from DNA extracted from DMSO-salt solution preserved tissues, whereas DNA from tissues stored in either lysis buffer or ethanol produced lower yields.     

Separation of outer and cytoplasmic membranes of Fibrobacter succinogenes and membrane and glycogen granule locations of glycanases and cellobiase.

The outer membrane (OM) of Fibrobacter succinogenes was isolated by a combination of salt, sucrose, and water washes from whole cells grown on either glucose or cellulose. The cytoplasmic membrane (CM) was isolated from OM-depleted cells after disruption with a French press. The OM and membrane vesicles isolated from the extracellular culture fluid of cellulose-grown cells had a higher density, much lower succinate dehydrogenase activity, and sodium dodecyl sulfate-polyacrylamide gel electrophoresis protein profiles different from those of the CM. The OM from both glucose- and cellulose-grown cells and the extracellular membrane vesicles from cellulose-grown cultures exhibited higher endoglucanase, xylanase, and acetylesterase activities than the CM and other cell fractions. Endoglucanase 2 was absent from the isolated OM fractions of glucose- and cellulose-grown cells and from the extracellular membrane vesicles of cellulose-grown cells but was present in the CM and intracellular glycogen granule fractions, while endoglucanase 3 was enriched in the OM. Cellobiosidase was located primarily in the periplasm as previously reported, while cellobiase was mainly present in the glycogen granule fraction of glucose-grown cells and in a nongranular glycogen and CM complex in cellulose-grown cells. The cellobiase was not eluted from glycogen granules by cellobiose, maltose, and maltotriose nor from either the granules or the cell membranes by nondenaturing detergents but was eluted from both glycogen granules and cell membranes by high concentrations of salts. The eluted cellobiase rebound almost quantitatively when diluted and mixed with purified glycogen granules but exhibited a low affinity for Avicel cellulose. Thus, we have documented a method for isolation of OM from F. succinogenes, identified the OM origin of the extracellular membrane vesicles, and located glycanases and cellobiase in membrane and glycogen fractions.