深海微生物高压适应与生物地球化学循环

深海是典型的高压环境,嗜压微生物是深海生态系统中的重要类群.随着深海采样技术的发展及高压微生物特殊培养设备的开发,已从深海环境中分离到一系列嗜压微生物,包括一些常压环境不能生长的严格嗜压菌.对这些嗜压菌的研究,不仅对微生物适应极端高压环境的机制有一定了解,而且发现了一些特殊的代谢产物.研究微生物高压嗜压机理,还有助于探索地球生命的温度压力极限及生命起源和演化等科学问题.从深海嗜压微生物多样性、深海微生物高压环境适应机理及深海微生物在生物地球化学循环中的作用等方面对嗜压微生物的研究进展进行综述.     

嗜酸硫杆菌在工农业中的应用

嗜酸硫杆菌(属)(Acidithiobacillus spp.)能够氧化亚铁、硫或还原性无机硫化合物(reduced inorganic sulfur compounds,RISCs)获得能量,固定二氧化碳,是一类典型的嗜酸性化能自养微生物。嗜酸硫杆菌广泛分布于酸性矿水、热泉等酸性环境中,是地球生态系统硫和铁元素循环的主要推动者。嗜酸硫杆菌独特的生理代谢特征和极端环境适应性,使其广泛应用于生物浸出领域。本文综述了嗜酸硫杆菌的生理代谢特征和极端环境下的适应机制,阐述了嗜酸硫杆菌在工农业中的应用,讨论了面向国家重大需求,嗜酸硫杆菌在今后的主要研究方向和需要解决的关键科学问题,为嗜酸硫杆菌在生理代谢、环境适应和工农业应用的研究提供重要的线索和启示。     

嗜盐古菌分类学研究进展

嗜盐古菌是一类需要高盐维持生长的古菌。到目前为止,已发现的嗜盐古菌都属于古菌域的广古菌门,主要包括:嗜盐甲烷古菌类群、嗜盐古菌纲的全部成员以及尚不能培养的纳米嗜盐古菌类群。嗜盐古菌是盐环境的土著类群,驱动着盐环境生态系统的生物地球化学循环。作为极端微生物,嗜盐古菌在理论研究和应用领域具有重要的研究价值。本文从嗜盐古菌分类学地位的变迁、分类学方法、分类学研究现状及我国的嗜盐古菌分类学研究等方面综述了嗜盐古菌分类学的最新研究进展。     

产嗜铁素砷抗性微生物在砷污染环境中的作用

在砷污染环境中,许多微生物进化出了砷抗性,对地球环境中砷的命运起着决定性的作用。其次,由于自然条件下铁有效浓度低,微生物一般会表达嗜铁素,协助微生物吸收铁。嗜铁素除了与铁结合外,还可与多种金属离子形成稳定的复合物,促进环境中砷酸盐的溶解和亚砷酸盐的氧化。最后,产嗜铁素微生物有促进植物生长和促进或减弱植物吸收砷的可能性。因此,产嗜铁素砷抗性微生物可能具有在砷污染环境的修复中发挥作用的潜力。     

极端微生物及其相关功能蛋白研究进展

极端微生物是一类能够适应特殊环境的微生物,相关功能蛋白在其适应极端环境过程中发挥着重要作用,探索极端微生物的特性及其相关的功能蛋白有助于深入了解生命的起源与进化,为蛋白酶在工业领域的应用提供一定理论依据。现概述耐辐射球菌、嗜盐菌、嗜热菌、嗜酸菌和嗜碱菌、嗜冷菌、嗜压菌的特性及其相关的功能蛋白质,从蛋白质水平阐述极端微生物对极端环境的适应机制。     

嗜盐放线菌分离方法

盐环境放线菌是一类独特的微生物资源。介绍了盐环境放线菌的种类,生理特性,影响嗜盐放线菌分离效果的基本因素,分离方法存在的问题,以及嗜盐放线菌分离的最新研究进展。推荐了3种适于分离嗜盐放线菌的培养基及分离方法。认为15%或以上NaCl浓度、一定比例的复合盐和培养基成分是高选择性分离嗜盐放线菌的关键。     

诱导选育嗜酸乳杆菌的鉴定

对亚硝基胍(NTG)诱变获得的嗜酸乳杆菌菌株的抗酸、抗胆盐及多项酶活力进行测定。亚硝基胍诱变的嗜酸乳杆菌培养于模拟胃肠环境的pH 3.5酸性环境90 min后,再培养于中性0.2%胆盐环境中,对其生长情况进行评估。对抗酸抗胆盐菌株的各项酶活性进行评估。嗜酸乳杆菌突变后筛选的2株菌株都具有良好的抗酸和抗胆盐能力,其中突变株Y48在模拟胃肠环境中生长良好,并具有良好的酶活性。诱变获得的优良嗜酸乳杆菌株,具有良好的抗酸抗胆盐及酶活各项性能,为开发优质的嗜酸乳杆菌新产品提供了条件。     

嗜酸菌耐酸pH平衡机制及潜在应用

嗜酸菌是一类可以在极端酸性环境下生存的微生物,在生物整治以及耐热耐酸酶的提取等领域发挥着重要作用。一些嗜中性工程菌株在发酵过程中经常遇到自身环境酸化的问题,嗜酸菌独特的耐酸能力及其耐酸模块为构建耐酸能力强的嗜中性工程菌株提供了思路。因此,从细胞膜的稳定性及低渗透性,耐酸相关的能量代谢,生物大分子的修复以及胞内缓冲作用等方面对嗜酸菌的耐酸机制进行深入探讨,并展望了嗜酸菌在耐酸工程菌株合成生物学领域的作用。     

碱性环境中的放线菌的生物学研究*

碱性环境中存在有一些嗜碱放线菌（Alkalophilic actinomycetes）,这些放线菌具有特殊的生理特征及代谢途径,可产生多种碱性酶及生物活性物质。综述了近20年来嗜碱放线菌的分类学研究,嗜碱菌的嗜碱机理,应用方面的研究进展,并展望了嗜碱放线菌的应用前景。     

微生物嗜盐酶的研究进展

嗜盐酶一般来自于嗜盐菌,它的主要特点是严格依赖体系中一定的盐离子浓度,可以在高盐环境中维持其结构稳定,并且能够抵抗高温、p H和有机溶剂存在下的变性,因此在高盐、水/有机和非水介质环境的催化中具有重要的应用价值。本综述从盐对嗜盐酶活性和稳定性的影响、金属离子和有机溶剂对嗜盐酶的影响几个方面介绍了嗜盐酶的特点。在总结蛋白质数据库(PDB)中已有嗜盐酶的结构和特点的基础上,对嗜盐酶的嗜盐机制进行了分析,认为嗜盐酶不同于非嗜盐酶的特点在于盐桥和氢键明显增多,含有一些特殊的盐离子结合位点并且常以低聚体的形式存在,表面酸性氨基酸含量明显增多。最后对嗜盐酶的分子改造和应用进行了简要的介绍。     

Comparative studies on thymidylate synthetase from P. berghei and mouse reticulocytes

Partially purified thymidylate synthetase from Plasmodium berghei and mouse reticulocytes was characterized. The mol. wt of the enzyme from P. berghei was about twice that from mouse reticulocytes. The optimum pH of the enzyme from P. berghei was found to be 6.5-7.5 while that from the host was 7.0-8.0. The enzyme from P. berghei was more susceptible to pH denaturation than the enzyme from reticulocytes. The enzyme from both sources differed in their Km values for substrates. The enzyme from reticulocytes was less sensitive to inhibition by substrate analogs than that from P. berghei.     

Influence of Indigenous Microbiota on Amount of Protein and Activities of Alkaline Phosphatase and Disaccharidases in Extracts of Intestinal Mucosa in Mice

The protein content and the activities of alkaline phosphatase, maltase, and sucrase were measured at 0800, 1000, 1200, 1400, and 1600 in saline extracts of the proximal small bowels of germfree and of ex-germfree mice colonized with an indigenous microbiota. In extracts prepared from germfree mice, the total activities of all of the enzymes were relatively constant throughout the sampling period. Likewise, the total activity of alkaline phosphatase in extracts prepared from associated mice varied little as a function of time. By contrast, the total activities of maltase and sucrase in the extracts from these latter animals varied significantly from sample to sample. The total activity levels in extracts from germfree mice were approximately twofold greater than the levels in extracts from associated mice. The specific activities of alkaline phosphatase and sucrase did not vary from sample to sample in extracts prepared from either type of mouse. In contrast, the specific activity of maltase in extracts prepared from both germfree and associated mice differed significantly from sample to sample. The specific activities of all three enzymes were greater in extracts from germfree animals than in those from associated animals. The protein content of extracts prepared from germfree mice also was greater than that of extracts prepared from associated animals at every sampling time. The amount of protein extractable from the mucosa of the small bowels of the former animals varied significantly at different sampling times during the day, whereas the amount of protein extractable from the tracts of associated animals remained relatively constant throughout the day. The indigenous microbiota apparently stabilizes in some way the amount of protein extractable from the mucosa of the mouse small bowel.     

The protein-synthesizing activity of ribosomes isolated from the mammary gland of lactating and pregnant guinea pigs

1. Polyribosome preparations were made from the deoxycholate-treated post-nuclear fractions obtained by the disruption of mammary glands from lactating and pregnant guinea pigs. 2. A high proportion of large polyribosomes was obtained from the glands of lactating animals whereas mainly small polyribosomes were obtained from the glands of pregnant animals. The isolated preparations incorporated [(14)C]phenylalanine into protein. The polyribosomes from the glands of pregnant animals were less active than those from the glands of lactating animals but the activity of the former was stimulated more by poly(U) than was the latter. 3. The ribosomes from mammary gland could be dissociated into subunits after incubation, under conditions necessary for protein synthesis, in the presence of puromycin. The subunits could be recombined to give a preparation that actively polymerized [(14)C]phenylalanine in the presence of poly(U). The subunits from guinea-pig mammary gland could be combined with subunits from liver of either guinea pig or rat. Hybrid ribosomes were also formed from subunits derived from glands of pregnant and lactating animals. The hybrids were as active as were the ribosomes formed by reassociation of subunits from the same tissue, suggesting that in this respect the ribosomes from pregnant animals were not defective. 4. Polyribosomes from mammary glands of lactating animals when incubated with cell sap from the same source were tested for their ability to synthesize alpha-lactalbumin. The polyribosomes were incubated in the presence of [(3)H]leucine and alpha-lactalbumin was isolated from the supernatant. The protein was finally treated with cyanogen bromide and the C-terminal and N-terminal fragments were separated and their radioactivity was determined. Both fragments were radioactive consistent with the synthesis of alpha-lactalbumin. 5. The results are discussed in relation to protein synthesis in the mammary gland after parturition.     

Development of microsatellite markers to genetically differentiate populations of Octopus minor from Korea and China

Of the more than 300 octopus species, Octopus minor is one of the most popular and economically important species in Eastern Asia, including Korea, along with O. vulgaris, O. ocellatus, and O. aegina. We developed 19 microsatellite markers from Octopus minor and eight polymorphic markers were developed to analyze the genetic diversity and relationships among four octopus populations from Korea and three from China. The number of alleles per locus varied from 10 to 49, and allelic richness per locus ranged from 2 to 16.4 across all populations. The average allele number among the populations was 11.1, with a minimum of 8.3 and a maximum of 13.6. The mean allelic richness was 8.7 in all populations. The Hardy-Weinberg equilibrium (HWE) test revealed significant deviation in 19 of the 56 single-locus sites, and null alleles were presumed in five of eight loci. The pairwise F ( ST ) values between populations from Korea and China differed significantly in all pairwise comparisons. The genetic distances between the China and Korea samples ranged from 0.161 to 0.454. The genetic distances among the populations from Korea ranged from 0.033 to 0.090, with an average of 0.062; those among populations from China ranged from 0.191 to 0.316, with an average of 0.254. The populations from Korea and China formed clearly separated into clusters via an unweighted pair group method with arithmetic mean dendrogram. Furthermore, a population from muddy flats on the western coast of the Korean Peninsula and one from a rocky area on Jeju Island formed clearly separated subclusters. An assignment test based on the allele distribution discriminated between the Korean and Chinese origins with 96.9 % accuracy.     

用SSR标记分析广西香稻与南亚香稻的遗传多样性

利用16对分布于水稻12条染色体上的SSR引物分析78份来自南亚的香稻资源和18份广西种植的香稻的遗传多样性。结果表明:在南亚的香稻资源中,每对引物检测到的等位基因数为3~13个,平均每个位点的等位基因数为5.31个,广西的香稻资源中,每对引物检测到等位基因数2~9个,平均每个位点的等位基因数为3.44个;南亚香稻资源平均多态信息含量(PIC)为0.55,广西香稻资源平均PIC为0.41;南亚香稻资源平均基因多样性(Hs)为0.60,广西香稻资源平均Hs为0.47;说明了南亚香稻资源比广西香稻资源具有更为丰富的遗传多样性。聚类结果表明,大部分的南亚香稻资源或大部分的广西香稻资源各自聚为一类,说明大部分南亚和广西的香稻种质资源存在遗传差异性和地理远缘性。     

Comparison of the nucleotide sequence of cloned DNA coding for an apolipoprotein (apoVLDL-II) from avian blood and the amino acid sequence of an egg-yolk protein (apovitellenin I): equivalence of the two sequences

We have compared the amino acid sequences of two low-molecular-weight avian apoproteins: apoVLDL-II from very low-density lipoproteins of hen plasma and apovitellenin I from hen egg yolk. The sequence of White Leghorn apoVLDL-II was derived from the nucleotide sequence of cloned apoVLDL-II DNA (Chan et al., 1980). The sequenator was used to determine the amino acid sequence of apovitellinin I from two breeds of hen (White Leghorn and Australorp). The sequences from the two breeds were not only identical, but they also completely matched the predicted sequence derived from the apoVLDL-II DNA sequence. The identity reported here establishes that this protein is transported intact from the blood to the egg yolk.     

The application of PCR fingerprinting to the differentiation of Yersinia enterocolitica strains isolated from humans and pigs

The distribution of different genotypes of Yersinia enterocolitica strains recovered from humans and from healthy pigs was investigated using PCR fingerprinting. The thirty six strains of Y. enterocolitica from humans, thirty five strains from pigs and Y. enterocolitica ATCC 9610 strain were included in this study. The tested strains of Y. enterocolitica belonged to O3 and O9 serogroups. The PCR fingerprinting using EAE5 primer (5' CTT AAT CTC AGT AAT GCT GGC CTT GG) made it possible to form five groups among the tested Y. enterocolitica strains. Two groups were very numerously represented by the tested strains. The thirty of Y. enterocolitica O3 strains from humans (thirty one of tested) and eighteen of Y. enterocolitica O3 strains from pigs (twenty of tested) belonged to one group. This group also included Y. enterocolitica ATCC9610 strain and four Y. enterocolitica O9 strains from pigs. All investigated Y. enterocolitica O9 strains from humans and the majority of Y. enterocolitica O9 strains isolated from pigs created a second, numerous group. The third genotype was created by two strains O9 from pigs, and the remaining two strains, isolated from pigs, belonging to O3 and O9 serogroups showed different binding patterns revealed by gel electrophoresis and created two other genotypes. The tested Y. enterocolitica strains which were isolated from humans formed only two groups but Y. enterocolitica strains isolated from pigs were found in five groups but such as the Y. enterocolitica strains from humans, the majority of strains from pigs were in first and second group. The Y. enterocolitica O3 strains regardless of their origin mostly represented the same PCR fingerprinting profile. The tested Y. enterocolitica O9 strains were more genetically diverse and represented four PCR fingerprinting profiles.     

Effects of vegetation change and soil disturbance on ectomycorrhizas ofBetula platyphylla var.japonica: A test using seedlings planted in soils taken from various sites

The occurrence and character of different types of ectomycorrhizas of birch seedlings were investigated in soils from three naturally regenerating birch stands: a forest site, a clear-cut site, and a site recently disturbed by plowing. Birch grown in soil from an evergreen broad-leaved forest without birch was also studied. The rate of ectomycorrhizal formation in the soil from the evergreen broad-leaved forest was lower than that in the soil from the other three sites. The ectomycorrhizal formation of seedlings grown in soil from the clear-cut and plowed sites were the same as or higher than that in soil from the birch forest site. The largest number of ectomycorrhizal types were formed in soil from the birch forest site. In the soil from the plowed site, only one type of ectomycorrhiza was formed, and it was different from the dominant type formed in soils from the birch forest site and the clear-cut site. The results of this investigation showed that equal levels of ectomycorrhizas were formed in soils from the different birch stands, but the types formed were different among those sites. It is likely that the different ectomycorrhizal fungi were better adapted to the soil conditions at each of those sites.     

Rabbit collagenase. Immunological identity of the enzymes released from cells and tissues in normal and pathological conditions.

1. The immunological cross-reactivity between rabbit collagenases from a variety of normal and pathological sources was examined. The specific antibody raised against collagenase secreted from normal rabbit synovial fibroblasts gave reactions of complete identity with collagenases secreted from fibroblasts derived from rabbit skin, and from synovium from experimentally arthritic rabbits. 2. The rabbit fibroblast collagenase was immunologically identical with collagenases obtained from the organ culture medium of normal rabbit skin, synovium, ear fibrocartilage and subchondral bone. 3. Collagenases from the culture media of normal rabbit synovium and from hyperplastic synovium of rabbits made experimentally arthritic were identical. 4. The collagenase secreted from rabbit fibroblasts gave a reaction completely identical with that of a collagenase extracted directly from a rabbit carcinoma. 5. IgG (immunoglobulin G) from a specific antiserum to rabbit fibroblast collagenase was a potent inhibitor of the collagenases obtained from the culture media of the various rabbit cells and tissues. 6. Collagenases from human synovium and from mouse macrophages and bone were neither precipitated nor inhibited by antibodies to rabbit collagenase. 7. No immunoreactive material was found in lysates of rabbit polymorphonuclear leucocyte granules with the specific antisera to rabbit fibroblast collagenase. No evidence for inactive forms of rabbit collagenase in lysates of the rabbit synovial fibroblasts could be found, either by double immunodiffusion against the specific collagenase, or by displacement of active enzyme from inhibition by the IgG.     

Regulation of ascorbic acid and of xylulose synthesis in liver extracts. The effect of starvation in various animals

1. The effect of starvation on the synthesis of ascorbic acid and of xylulose from glucuronolactone and from gulonate has been studied with liver extracts from cats, rabbits, hamsters, mice and guinea pigs. 2. The synthesis of ascorbic acid from glucuronolactone is decreased in all species except cats, and that from gulonate is decreased in hamsters and mice only. 3. The synthesis of xylulose from glucuronolactone was decreased in all species except cats and mice, whereas from gulonate it was enhanced in all the species examined.