千层塔中产石杉碱甲内生真菌的研究

从千层塔中分离产石杉碱甲内生真菌。采用平板分离法分离千层塔内生真菌,通过抑制乙酰胆碱酯酶活性和抗氧化活性筛选,结合薄层层析和HPLC测定活性菌株中的石杉碱甲含量,通过形态学ITS-rDNA序列分析鉴定内生真菌。共分离得到94株内生真菌,筛选到S29、L44、S94共3株乙酰胆碱酯酶抑制活性和清除DPPH·自由基活性都在50%以上,筛选到一株S29能产石杉碱甲的菌株。摇瓶发酵产量为每克干菌体的石杉碱甲含量为50.64μg。形态学与ITS-rDNA序列分析法鉴定该内生真菌为Podospora sp.属。药用植物千层塔体内Podospora sp.属的内生真菌可产石杉碱甲。     

蛇足石杉中产石杉碱甲内生真菌的分离和鉴定

【目的】从野生蛇足石杉(Huperzia serrata)中分离筛选产石杉碱甲的内生真菌。【方法】采用薄层层析及高效液相色谱法对内生真菌代谢产物进行测定和分析以期分离获得产石杉碱甲菌株,运用形态及ITS序列分析方法对产石杉碱甲菌株进行鉴定,并利用连续传代方法考察菌株遗传稳定性。【结果】经筛选获得一株产石杉碱甲内生真菌NSH-5,经形态学鉴定及ITS序列分析鉴定为轮枝镰孢菌(Fusarium verticillioides),其石杉碱甲产量为11.76 mg/100 m L,菌株经20次连续传代后遗传稳定。【结论】NSH-5菌株为一株具有产石杉碱甲能力的轮枝镰孢菌,该菌株的发现为生物合成石杉碱甲提供了新的菌种资源。     

蛇足石杉产石杉碱甲内生真菌SNZ-12的分离及鉴定北大核心CSCD

为了获取具有应用价值的产石杉碱甲内生菌,本文从蛇足石杉分离得到60株内生真菌,采用高效液相色谱法和质谱法分别检测各个真菌的提取物,发现内生真菌SNZ-12的提取物具有与石杉碱甲标品相近的色谱特征峰和保留时间(8. 994 min)以及相同的质谱特征峰((M+H)+=243. 1),说明内生真菌SNZ-12可以产石杉碱甲,其石杉碱甲产量约为1. 01 mg/L;并通过结合内生真菌SNZ-12的形态特征和18S r DNA序列分析,将其鉴定为尖孢镰刀菌(Fusarium oxysporum)。本文结果为利用微生物发酵生产石杉碱甲研究提供了潜在的菌种资源。     

蛇足石杉产石杉碱甲内生真菌SNZ-12的分离及鉴定

为了获取具有应用价值的产石杉碱甲内生菌,本文从蛇足石杉分离得到60株内生真菌,采用高效液相色谱法和质谱法分别检测各个真菌的提取物,发现内生真菌SNZ-12的提取物具有与石杉碱甲标品相近的色谱特征峰和保留时间(8. 994 min)以及相同的质谱特征峰((M+H)+=243. 1),说明内生真菌SNZ-12可以产石杉碱甲,其石杉碱甲产量约为1. 01 mg/L;并通过结合内生真菌SNZ-12的形态特征和18S r DNA序列分析,将其鉴定为尖孢镰刀菌(Fusarium oxysporum)。本文结果为利用微生物发酵生产石杉碱甲研究提供了潜在的菌种资源。     

HPLC法检测蛇足石杉内生真菌胶胞炭疽发酵液中石杉碱甲和石杉碱乙的含量

建立了高效液相色谱(HPLC)测定蛇足石杉(Huperzia serrate)内生真菌胶胞炭疽发酵液中石杉碱甲(Huperzina A)和石杉碱乙(Huperzine B)含量的方法,并以此方法检测胶胞炭疽发酵液中石杉碱甲和石杉碱乙含量的积累。内生真菌发酵液经氯仿萃取、甲醇溶解、过滤后进行高效液相检测分析,选用Agilent Eclipse plus-C18色谱柱(250 mm×4.6 mm,5μm),以0.015 mol/L乙酸铵(p H 6.8)和甲醇溶液(70∶30)为流动相进行等度洗脱,流速1 mL/min,检测波长为308 nm,连续检测内生真菌胶胞炭疽发酵液中第6–15天石杉碱甲和石杉碱乙的含量积累。结果表明,发酵提取液中的石杉碱甲和石杉碱乙可在25 min内进行很好的分离和分析,石杉碱甲在1.50-48.00μg/mL范围内线性关系良好(相关系数r为0.999 5),石杉碱乙在0.25-7.50μg/mL范围内线性关系良好(相关系数r为0.999 7),石杉碱甲和石杉碱乙的平均加标回收率分别为106.83%、108.06%,相对标准偏差(RSD)分别为3.34%、3.60%。该方法简便、快速、精密度高、结果准确,适用于内生真菌发酵液中石杉碱甲和石杉碱乙含量检测。在发酵过程中,内生真菌发酵液中石杉碱甲和石杉碱乙的含量呈现先增后减,随后有所增加继而又减少的趋势。石杉碱甲和石杉碱乙的含量分别在内生真菌发酵第14天、第8天达到最高,分别为12.417 0μg/mL、4.660 3μg/mL。该方法学的建立为内生真菌胶胞炭疽合成石杉碱甲与石杉碱乙的机制研究提供了检测手段,从而有利于药物新资源的开发。     

一株产石杉碱甲的蛇足石杉内生真菌的分离和鉴定

从药用蕨类植物蛇足石杉叶中分离得到53株内生真菌,在马铃薯葡萄糖液体培养基（PDB）中发酵后对内生真菌发酵提取物液进行TLC、HPLC 和ESI-MS检测,结果表明菌株LF40为产石杉碱甲内生菌株,含量达80.1μg/gdcw,并具有体外乙酰胆碱酯酶抑制活性;运用形态学及ITS-rDNA序列分析方法对菌株LF40进行鉴定,确定为黄曲霉Aspergillus flavus LF40。     

从蛇足石杉中超声提取石杉碱甲和石杉碱乙

用正交试验确立了超声提取蛇足石杉生物碱的最佳条件。以石杉碱甲和石杉碱乙回收率为指标,考察了溶剂倍数、溶剂浓度、超声时间、超声功率等因素的影响。结果表明,在室温下超声提取的最优条件为：酸浓度O．8％(v／v),液固比例20：1,超声功率600W,超声15min。三次重复实验所得石杉碱甲和石杉碱乙回收率分别是9r7．3％和93．5％,相对标准偏差分别为1．31％和1．40％(n=3)。与传统的回流提取工艺相比,过程时间从2h缩短为15min,回收率提高了10％以上。     

白腐真菌AH28-2菌株发酵合成漆酶初步研究

从224个野外采集的真菌样品中筛选分离到一株产漆酶活性较高菌株AH28－2,经初步鉴定为白腐真菌,采用单因子相互比较法,研究了该菌株最适发酵产酶条件。应用添加有1g／LKraft木素的液体发酵培养基,接种量5％（V／V）,初始pH8．5,装液量为50％,28℃、150r/min摇瓶振荡培养4－5d,漆酶酶活水平达20184IU／L。     

蛇足石杉产石杉碱甲内生真菌的分离鉴定

从9月份采集的野生药用植物蛇足石杉(Huperzia serrata)的茎、叶中分离纯化得到15株内生真菌,将上述内生真菌进行液体培养后,通过薄层层析法(TLC)和高效液相法(HPLC)对其代谢产物进行检测,结果表明菌株WX13产石杉碱甲(Huperzine A,HupA)。运用形态和培养特性观察,初步确定菌株WX13属于镰刀菌属(Fu-sarium sp.)。     

最新专利文摘

CN102653720A 一株产石杉碱甲的蛇足石杉内生真菌ES026 本发明公开了一株从药用植物蛇足石杉中分离出的内生真菌。本发明分离的内生真菌ES026经分子生物学和形态学鉴定为炭疽属胶孢种（Colletotrichum gloeosporioides）,该菌株已保藏在中国典型培养物保藏中心,保藏编号为CCTCCM2011046。     

Invasion pathway of the honeybee pest,small hive beetle,Aethina tumida (Coleoptera: Nitidulidae) in the Republic of Korea inferred by mitochondrial DNA sequence analysis

The small hive beetle (SHB), Aethina tumida, is native to the Sub-Saharan region of Africa, but it became invasive in many countries after its first introduction to the USA in 1996. The SHB is a destructive pest of the honey industry and can cause damage in apiaries due to feeding on the honey, pollen, honey bee brood and honey fermentation. SHB was recently found infesting honeybee colonies in the South-Eastern part of Korea, Miryang city in 2016. No inference of the origin or the pathway of the invasion into Korea has been made, so far. We analyzed partial cytochrome oxidase I gene of mitochondrial DNA to unveil the possible source of the invasive populations of SHB in South Korea. A Bayesian inference tree and median joining haplotype network revealed a strong relationship between South Korean and North American populations suggesting that the SHB in South Korea came from the USA. Low genetic variation among Korean populations suggests that the invasion might have occurred in a single event with small number of founders. In addition, a new global distributional map of SHB is provided.     

The FRK/RAK-SHB signaling cascade: a versatile signal-transduction pathway that regulates cell survival,differentiation and proliferation

Recent experiments have unravelled novel signal transduction pathways that involve the SRC homology 2 (SH2) domain adapter protein SHB. SHB is ubiquitously expressed and contains proline rich motifs, a phosphotyrosine binding (PTB) domain, tyrosine phosphorylation sites and an SH2 domain and serves a role in generating signaling complexes in response to tyrosine kinase activation. SHB mediates certain responses in platelet-derived growth factor (PDGF) receptor-, fibroblast growth factor (FGF) receptor-, neural growth factor (NGF) receptor TRKA-, T cell receptor-, interleukin-2 (IL-2) receptor- and focal adhesion kinase- (FAK) signaling. Upstream of SHB in some cells lies the SRC-like FYN-Related Kinase FRK/RAK (also named BSK/IYK or GTK). FRK/RAK and SHB exert similar effects when overexpressed in rat phaeochromocytoma (PC12) and beta-cells, where they both induce PC12 cell differentiation and beta-cell proliferation. Furthermore, beta-cell apoptosis is augmented by these proteins under conditions that cause beta-cell degeneration. The FRK/RAK-SHB responses involve FAK and insulin receptor substrates (IRS) -1 and -2. Besides regulating apoptosis, proliferation and differentiation, SHB is also a component of the T cell receptor (TCR) signaling response. In Jurkat T cells, SHB links several signaling components with the TCR and is thus required for IL-2 production. In endothelial cells, SHB both promotes apoptosis under conditions that are anti-angiogenic, but is also required for proper mitogenicity, spreading and tubular morphogenesis. In embryonic stem cells, dominant-negative SHB (R522K) prevents early cavitation of embryoid bodies and reduces differentiation to cells expressing albumin, amylase, insulin and glucagon, suggesting a role of SHB in development. In summary, SHB is a versatile signal transduction molecule that produces diverse biological responses in different cell types under various conditions. SHB operates downstream of GTK in cells that express this kinase.     

Application of L-Amino acid in determination of Huperzine A by high performance liquid chromatography

A selective HPLC method for determination of Huperzine A in Huperzia serrata Extract has been developed and validated. Huperzine A was dissolved in 0.01 mol/L HCl, chromatographed on an Agilent Zorbax SB-C18 (150 mm x 4.6 mm i.d., 5 microm) column, with a mobile phase consisting of methanol-1mM L-Lysine water solution (50:50, v/v), and detected at 310 nm. The UV peak areas were used for quantitation of Huperzine A content. The correlation coefficient (R(2)) of the calibration was 0.9999 over the range of 1-25 microg/ml and intra- and interday precision over this range were not more than 2%. The method was successfully applied to characterize and determine the Huperzine A in Huperzia serrata Extract.     

Production and isolation of chitosan by submerged and solid-state fermentation from Lentinus edodes

A method for the laboratory-scale production and isolation of chitosan (polyglucosamine) by liquid and solidstate fermentation from Lentinus edodes was developed. The yields of isolated chitosan were 120 mg/L of fermentation medium under liquid fermentation conditions and 6.18 g/kg of fermentation medium under solid-state fermentation conditions. The latter method, which gives up to 50 times yields than other chitosan production methods from fungi, provides a new flexible and easily scaledup procedure for the production of low acetylation degree chitosan. (c) 1996 John Wiley & Sons, Inc.     

乙型肝炎病毒小表面抗原各拓扑区段对其表达和分泌的影响

乙型肝炎病毒小表面抗原(small hepatitis B virus surface antigen,SHB)在细胞内质网上表达,沿着细胞分泌途径分泌到胞外。为系统分析SHB拓扑结构对SHB表达和分泌的影响,首先通过生物信息学预测临床病毒株HBV C8和8种基因型(A~H)代表株的SHB拓扑结构,发现这些SHB均为四次跨膜蛋白,拥有基本相同的拓扑结构。相对内质网膜而言,SHB的拓扑结构拥有3个内质网腔内区段(Inside1~Inside3)、4个跨膜螺旋区(Tmhelix1~Tmhelix4)和2个内质网膜外区段(Outside1和Outside2)。6种基因型(基因型A、B、C、D、E和G)代表株与病毒株C8的SHB拓扑结构预测结果完全相同,而基因型F和H的SHB有4个区段与C8等不完全一致。通过对C8的SHB拓扑结构各区段进行缺失突变研究,发现Inside1区段不是SHB表达和分泌所必需的;Outside1、Tmhelix2和Inside2区段是SHB表达和分泌所必需的;Tmhelix1和Outside2不是SHB表达所必需的,但为SHB分泌所必需;Tmhelix3和Tmhelix4对SHB表达有重要影响,也是SHB分泌所必需的。进一步对Outside1和Outside2进行小片段(6个氨基酸)的缺失突变研究,发现小片段缺失基本不显著影响SHB的表达,但Outside1的氨基酸55~78及Outside2是SHB分泌所必需的。本研究首次系统性分析了SHB的拓扑结构各区段对SHB表达和分泌的影响,为深入探索SHB结构与功能的关系提供了线索。     

一株高产洛伐他汀红曲霉的筛选与液态发酵条件优化

【背景】洛伐他汀(lovastatin)是红曲霉的次生代谢产物,是重要的临床用降血脂药物。在液态发酵条件下,红曲霉的洛伐他汀产量较低,难以满足工业化生产的要求。【目的】筛选获得一株高产洛伐他汀的红曲霉株,并通过优化液态发酵条件提高洛伐他汀的产量。【方法】从红曲米中筛选获得一株高产洛伐他汀的红曲霉株,依据形态学特征、生理生化特性及18S rRNA基因序列分析对分离菌株进行鉴定;通过响应面法对其产洛伐他汀的液态发酵条件进行优化。【结果】获得一株产洛伐他汀的紫红曲霉(Monascus purpureus M4),该菌在甘油57.80g/L、酵母浸粉5.52 g/L、接种量为6.90%条件下,洛伐他汀产量(173.60 mg/L)较优化前提高了4.8倍。【结论】菌株M4产洛伐他汀最优液态发酵条件的建立,为洛伐他汀的大规模生产及该菌株的工业化应用提供了技术支撑。     

Global analysis of canola genes targeted by SHORT HYPOCOTYL UNDER BLUE 1 during endosperm and embryo development

Seed development in dicots includes early endosperm proliferation followed by growth of the embryo to replace the endosperm. Endosperm proliferation in dicots not only provides nutrient supplies for subsequent embryo development but also enforces a space limitation, influencing final seed size. Overexpression of Arabidopsis SHORT HYPOCOTYL UNDER BLUE1::uidA (SHB1:uidA) in canola produces large seeds. We performed global analysis of the canola genes that were expressed and influenced by SHB1 during early endosperm proliferation at 8 days after pollination (DAP) and late embryo development at 13 DAP. Overexpression of SHB1 altered the expression of 973 genes at 8 DAP and 1035 genes at 13 DAP. We also surveyed the global SHB1 association sites, and merging of these sites with the RNA sequencing data identified a set of canola genes targeted by SHB1. The 8‐DAP list includes positive and negative genes that influence endosperm proliferation and are homologous to Arabidopsis MINI3, IKU2, SHB1, AGL62, FIE and AP2. We revealed a major role for SHB1 in canola endosperm development based on the dynamics of SHB1‐altered gene expression, the magnitude of SHB1 chromatin immunoprecipitation enrichment and the over‐representation of eight regulatory genes for endosperm development. Our studies focus on an important agronomic trait in a major crop for global agriculture. The datasets on stage‐specific and SHB1‐induced gene expression and genes targeted by SHB1 also provide a useful resource in the field of endosperm development and seed size engineering. Our practices in an allotetraploid species will impact similar studies in other crop species.     

Olfactory responses of Aethina tumida murray (Coleoptera: Nitidulidae) to some major volatile compounds from hive materials and workers of Apis mellifera

The small hive beetle (Aethina tumida Murray) is an invasive pest affecting honey bee colonies. The beetles are known to be attracted to volatiles from hive products and honey bees like Apis mellifera L. Previously we reported the presence of five major compounds from the volatile extracts of hive materials; ethyl linolenate and ethyl palmitate from pollen dough, oleamide and tetracosane in fermenting honey, and oleamide and 5-methyl-2-phenyl-1H-indole from A. mellifera worker bees. This study tested the attractiveness of the aforementioned five volatile organic compounds to small hive beetles (SHB) by Y-tube olfactometric bioassay. Ethyl linolenate was highly attractive to both male and female adults of SHB. Ethyl palmitate was attractive to SHB only at higher concentration (0.01–01 mg/ml). Interestingly, tetracosane, 5-methyl-2-phenyl-1H-indole and oleamide were repellent for SHB of both sexes, but ethyl linolenate and ethyl palmitate as components of honey bee brood pheromone attracted SHB. The results highlight that SHB differentially utilizes volatile chemicals from hive materials and honey bees as cues to locate honey bee hives.     

Huperzine A Ameliorates Cognitive Deficits and Oxidative Stress in the Hippocampus of Rats Exposed to Acute Hypobaric Hypoxia

Acute exposure to high altitudes can cause neurological dysfunction due to decreased oxygen availability to the brain. In this study, the protective effects of Huperzine A on cognitive deficits along with oxidative and apoptotic damage, due to acute hypobaric hypoxia, were investigated in male Sprague–Dawley rats. Rats were exposed to simulated hypobaric hypoxia at 6,000 m in a specially fabricated animal decompression chamber while receiving daily Huperzine A orally at the dose of 0.05 or 0.1 mg/kg body weight. After exposure to hypobaric hypoxia for 5 days, rats were trained in a Morris Water Maze for 5 consecutive days. Subsequent trials revealed Huperzine A supplementation at a dose of 0.1 mg/kg body weight restored spatial memory significantly, as evident from decreased escape latency and path length to reach the hidden platform, and the increase in number of times of crossing the former platform location and time spent in the former platform quadrant. In addition, after exposure to hypobaric hypoxia, animals were sacrificed and biomarkers of oxidative damage, such as reactive oxygen species, lipid peroxidation, lactate dehydrogenase activity, reduced glutathione, oxidized glutathione and superoxide dismutase were studied in the hippocampus. Expression levels of pro-apoptotic proteins (Bax, caspase-3) and anti-apoptotic protein (Bcl-2) of hippocampal tissues were evaluated by Western blotting. There was a significant increase in oxidative stress along with increased expression of apoptotic proteins in hypoxia exposed rats, which was significantly improved by oral Huperzine A at 0.1 mg/kg body weight. These results suggest that supplementation with Huperzine A improves cognitive deficits, reduces oxidative stress and inhibits the apoptotic cascade induced by acute hypobaric hypoxia.     

深海细菌SHB109的鉴定及其表面活性产物研究

从南海深海海泥中分离得到1株海洋细菌SHB109.采用形态学鉴定方法,并结合16S rDNA序列分析确定其为枯草芽胞杆菌斯皮兹亚仁亚种(Bacillus subtilis subsp.spizizenii).从其发酵液中分离得到3个化合物,通过1 H-NMR,13C-NMR及HR ESI MS光谱分析将它们鉴定为sur...