羧甲基茯苓多糖抗疲劳作用研究

研究羧甲基茯苓多糖(CMP)对小鼠抗疲劳作用。将雄性小鼠随机分为5组,分别为空白对照组、阳性对照组、CMP低剂量组(35 mg/(kg bw·d))、CMP中剂量组(70 mg/(kg bw·d))、CMP高剂量组(140 mg/(kg bw·d)),灌胃给药30 d后,测定小鼠负重的游泳时间、血清尿素氮和血乳酸等指标。结果表明,与空白对照组相比,CMP可以延长小鼠负重游泳时间(P0.05);CMP中、高剂量组可以显著降低血清尿素氮、血乳酸含量并提高肝脏SOD活性(P0.05)。CMP对小鼠具有很好的抗疲劳作用,其机制可能与降低血清尿氮素、血乳酸含量以及提高肝脏SOD活性有关。     

羧甲基茯苓多糖的制备及体内抗肿瘤作用的实验研究

目的 :探讨羧甲基茯苓多糖的制备方法及体内抗肿瘤作用。方法 :选择性氧化茯苓菌发酵液得羧甲基茯苓多糖 ,检测三个剂量的羧甲基茯苓多糖 (2 mg/ ml、4mg/ ml、6mg/ ml)对 H2 2 荷瘤小鼠淋巴细胞转化率和 NK细胞杀伤活性以及血清中 TNF-α含量的影响。结果 :羧甲基茯苓多糖三个剂量组均可提高荷瘤小鼠的淋巴细胞转化率和 NK细胞杀伤活性 ,与生理盐水组相比差异有显著性 (P<0 .0 5) ,中剂量组抗肿瘤的效果显著 ,与其他两组相比差异有显著性 (P<0 .0 5) ;羧甲基茯苓多糖三个剂量组均可提高荷瘤小鼠血清中 TNF-α的含量 ,与生理盐水组相比差异有显著性 (P<0 .0 5) ,但三个剂量组之间比较差异无显著性 (P<0 .0 5)。结论 :羧甲基茯苓多糖可改善荷瘤小鼠的免疫功能 ,具有抗肿瘤作用 ,且功效与作用剂量间有一定的关系 ,在最佳剂量时活性最高     

羧甲基茯苓多糖体外抗氧化活性研究

目的：比较不同浓度洗脱液洗脱得到的羧甲基茯苓多糖的抗氧化活性。方法：以茯苓为原料提取茯苓多糖,进行羧甲基取代反应,分离和纯化得到了均一性羧甲基茯苓多糖CMP-1、CMP-2、CMP-3、CMP-4,通过测定还原能力、DPPH自由基清除率、羟基自由基清除率、超氧阴离子自由基清除率比较其体外抗氧化活性。结果：羧甲基茯苓多糖均表现出与浓度正相关的体外抗氧化活性,其中CMP-4具有相对更强的体外抗氧化活性。结论：所得羧甲基茯苓多糖样品具有不同的体外抗氧化能力,随着洗脱液浓度增加,抗氧化活性增强。     

不同组分羧甲基茯苓多糖（CMP）对HepG2细胞增殖的影响

目的：探究不同组分羧甲基茯苓多糖（CMP）对HepG2细胞增殖的影响。方法：在不同提取碱浓度和碱处理时间下,采用二次加碱法制备不同组分CMP。利用硫酸 蒽酮法、滴定法和CCK 8法对CMP的含量、取代度和HepG2细胞增殖检测。结果：获得7个组分CMP,含量为85%~90 %,取代度为0.65~0.80。不同浓度CMP培养HepG2细胞24 h下,CMP 750 μg/mL抑制细胞增殖效果最好,其中CMP3抑制率最高达50.035 %。CMP 750 μg/mL培养HepG2细胞24、48、72 h,在48 h下抑制效果最好,其中CMP3抑制效果最高达到76.05 %。在72、48、24 h 下CMP3培养HepG2细胞的IC50分别为26.34、34.06、763.64 μg/mL。结论：CMP能有效抑制HepG2肿瘤细胞的增殖,其中CMP3是7个CMP组分中抑制效果最好的,这与CMP3的含量、浓度呈正相关性,48 h为CMP最适抑制时间。     

液体发酵茯苓胞外多糖的体外降糖效果研究

为探究液体发酵茯苓胞外多糖的体外降糖效果,本研究以高胰岛素抵抗HepG2细胞为受试对象,分析了不同浓度的茯苓胞外多糖对葡萄糖消耗、细胞增殖和糖原合成的影响,并考察了茯苓胞外多糖对α-葡萄糖苷酶的抑制活性。研究结果显示,茯苓胞外多糖可显著促进高胰岛素抵抗HepG2细胞的葡萄糖消耗(p0.05),并加速其糖原合成,但对其细胞增殖无抑制活性;此外,茯苓胞外多糖在终浓度高于2.5μg/mL时还可表现出显著的α-葡萄糖苷酶抑制活性,最大抑制率可达29.51%。研究表明,液体发酵茯苓胞外多糖具有非常好的体外降糖效果。     

真菌多相结构的化学修饰

真菌多糖因具有独特的分子结构,一般都具有促进免疫、抑制肿瘤的活性,但这种活性随真菌种类及其产生的多糖种类不同而差异较大;另外真菌多糖都具有较大的分子量,水中溶解性较差,这为真菌多糖的实际应用造成了一定的困难．对某些真菌多糖的结构进行必要的化学修饰,不仅可增强其促进免疫和抗肿瘤活性,而且水溶性也大大地提高。茯苓多糖是β-1,6-葡糖链分支的β-1,3-葡聚糖,没有抗肿瘤活性,经高碘酸氧化、Smith降解、硼氢化钠还原可得较小分支的中间产物,再经酸水解去除分支得到直链多糖,即茯苓新糖。茯苓新糖和中间产物均具有很…     

A群奈瑟氏脑膜炎球菌荚膜多糖-破伤风类毒素结合疫苗的制备及其免疫原性研究

采用溴化氰(CNBr)活化多糖,以无水己二酸二肼(ADH)作为连接剂,1乙基13(3二甲基氨基丙基)碳化二亚胺(EDAC)为偶联剂制备A群奈瑟氏脑膜炎球菌荚膜多糖(GAMP)与破伤风类毒素(TT)的结合物,经皮下免疫NIH小鼠,用ELISA检测小鼠血清中抗GAMP及抗载体蛋白的IgG抗体水平。用补体介导的体外杀菌试验检测血清中GAMP抗体的杀菌活性。结果显示,实验中制备的多糖衍生物和多糖蛋白质结合物都具有GAMP抗原特异活性。结合物免疫小鼠后可诱生比多糖单独免疫更高水平的GAMP血清IgG抗体,并能形成免疫记忆,产生再次应答。结合物免疫小鼠所诱生的血清GAMP抗体较之多糖组具有更强的体外杀菌活性。表明此方法制备的结合物可获得优于多糖的、稳定的特异免疫原性。     

一种牛樟芝深层发酵复方制品的制备方法研究

目的探讨一种牛樟芝深层发酵复方制品的制备方法。方法选择以茯苓粉、山药粉、葛根粉、蜂花粉、大豆粉等原料配制深层发酵培养基,经深层发酵培养富含牛樟芝多糖的牛樟芝菌丝体发酵液,与采用超临界CO2技术提取、酶解、分离、过滤、浓缩制得的佛手、黄精、枸杞、砂仁、余甘子、枳椇子等中草药提取液复合。结果配制为一种牛樟芝深层发酵复方制品。结论该方法优化了牛樟芝多糖等活性成分的含量,具有产量高、时间短、成本低,可以工业化生产,而且高效环保,具有开发应用前景。     

茯苓多糖抗氧化性研究

采用分光光度法研究了茯苓多糖提取物的体外抗氧化作用,并与Vc进行比较.结果表明其具有较强的抗氧化能力,在清除DPPH·的体系中和还原能力体系中,样品的清除能力均超过Vc,但在羟基自由基·OH和超氧阴离子O-2体系中,其清除能力低于对照样Vc.     

发酵茯苓菌丝体和天然茯苓多糖的研究

本文对发酵茯苓菌丝体和天然茯苓中多糖的提取分离进行了研究,并分别测定了二者总多糖的提取率及总糖的平均含量。发酵茯苓菌丝体和天然茯苓中总多糖的提取率分别为24.47%和82.93%;发酵茯苓菌丝体和天然茯苓总糖的平均含量分别为45.17%和87.24%。     

Optimization of the Extraction Process and Antioxidant Activity of Polysaccharide Extracted from Centipeda minima

The purpose of this study is to optimize the extraction process and study antioxidant activity of Polysaccharide extracted from Centipeda minima. The Box-Behnken design-response surface methodology was adopted to optimize the extraction process of polysaccharides from Centipeda minima. We purified the crude polysaccharides from Centipeda minima, as well as determined the purity, monosaccharide composition, and molecular weight of the purified fraction. Fourier transform infrared spectrometer (FT-IR) and scanning electron microscopy (SEM) were used to analyze the structural features of the polysaccharides. Further, we investigated the antioxidant activities of different fractions of polysaccharides. Consequently, the results showed that the optimum extraction conditions for polysaccharides were: a liquid-solid ratio of 26 mL/g, extraction temperature of 85.5 °C, and extraction time of 2.4 h. Moreover, the yield of polysaccharides measured under these conditions was close to the predicted value. After purification, we obtained four components of Centipeda minima polysaccharides (CMP). The purity, monosaccharide composition, molecular weight, and structural characteristics of CMP were different, but with similar infrared absorption spectra. CMP exhibited a typical infrared absorption characteristic of a polysaccharide. Besides, CMP displayed good antioxidant activity, with potential to scavenge DPPH radical, hydroxyl radical, and superoxide radical. Therefore, this study provides a reference for future research on the structure and biological activity of CMP, and lays a theoretical foundation for food processing and medicinal development of CMP.     

Functionalization of magnetic nanowires by charged biopolymers

We report on a facile method for the preparation of biocompatible and bioactive magnetic nanowires. The method consists of the direct deposition of polysaccharides by layer-by-layer (LbL) assembly onto a brush of metallic nanowires obtained by electrodeposition of the metal within the nanopores of an alumina template supported on a silicon wafer. Carboxymethylpullulan (CMP) and chitosan (CHI) multilayers were grown on brushes of Ni nanowires; subsequent grafting of an enzyme was performed by conjugating free amine side groups of chitosan with carboxylic groups of the enzyme. The nanowires are finally released by a gentle ultrasonic treatment. Transmission electron microscopy, electron energy-dispersive loss spectroscopy, and x-ray photoelectron spectroscopy indicate the formation of an homogeneous coating onto the nickel nanowires when one, two, or three CMP/CHI bilayers are deposited. This easy and efficient route to the biochemical functionalization of magnetic nanowires could find widespread use for the preparation of a broad range of nanowires with tailored surface properties.     

Cytidine 5'-monophosphate (CMP)-induced structural changes in a multifunctional sialyltransferase from Pasteurella multocida

Sialyltransferases catalyze reactions that transfer a sialic acid from CMP-sialic acid to an acceptor (a structure terminated with galactose, N-acetylgalactosamine, or sialic acid). They are key enzymes that catalyze the synthesis of sialic acid-containing oligosaccharides, polysaccharides, and glycoconjugates that play pivotal roles in many critical physiological and pathological processes. The structures of a truncated multifunctional Pasteurella multocida sialyltransferase (Delta24PmST1), in the absence and presence of CMP, have been determined by X-ray crystallography at 1.65 and 2.0 A resolutions, respectively. The Delta24PmST1 exists as a monomer in solution and in crystals. Different from the reported crystal structure of a bifunctional sialyltransferase CstII that has only one Rossmann domain, the overall structure of the Delta24PmST1 consists of two separate Rossmann nucleotide-binding domains. The Delta24PmST1 structure, thus, represents the first sialyltransferase structure that belongs to the glycosyltransferase-B (GT-B) structural group. Unlike all other known GT-B structures, however, there is no C-terminal extension that interacts with the N-terminal domain in the Delta24PmST1 structure. The CMP binding site is located in the deep cleft between the two Rossmann domains. Nevertheless, the CMP only forms interactions with residues in the C-terminal domain. The binding of CMP to the protein causes a large closure movement of the N-terminal Rossmann domain toward the C-terminal nucleotide-binding domain. Ser 143 of the N-terminal domain moves up to hydrogen-bond to Tyr 388 of the C-terminal domain. Both Ser 143 and Tyr 388 form hydrogen bonds to a water molecule, which in turn hydrogen-bonds to the terminal phosphate oxygen of CMP. These interactions may trigger the closure between the two domains. Additionally, a short helix near the active site seen in the apo structure becomes disordered upon binding to CMP. This helix may swing down upon binding to donor CMP-sialic acid to form the binding pocket for an acceptor.     

Preparation and properties of fluorescent polysaccharides

A new method for preparing fluorescein derivatives of polysaccharides is described. These derivatives are prepared by activation of the polysaccharide with cyanogen bromide and subsequent reaction with fluoresceinamine. The optimum conditions for coupling have been established in this report. Using this procedure, we have prepared fluorescein derivatives of a wide variety of polysaccharides. Degrees of substitution in the range of 3.0 X 10(-3) to 2.4 X 10(-2) mol of fluorescein per mole of monosaccharide equivalent were obtained. The fluorescent derivatives are stable: no free fluorescein was detected after incubation at 22 degrees C for 48 h or at -10 degrees C for 4 months. The fluorescein-derivatized polysaccharides were found to have the same potency in inhibiting lectin-mediated hemagglutination as the underivatized polysaccharide. In addition, these fluorescent polysaccharides can be radioiodinated to specific activities exceeding 10(6) dpm/micrograms due to incorporation of 125I into fluorescein. The cell binding properties of 125I-fucoidin and 125I-heparin are indistinguishable from the corresponding underivatized polysaccharides. This general approach for preparing fluorescent polysaccharides should produce useful reagents for localizing and quantifying cell surface carbohydrate-binding proteins (lectins).     

Quantitation of Cytidine 3′,5′-Cyclic Monophosphate in Aqueous Solution by UV Absorption Spectrophotometry Independent of Direct Determination of Solution pH

Abstract

uv absorbance spectrophotometry is the routine method of determining nucleotide concentrations in solution. To obviate the need for determining solution pH a method is described whereby cyclic CMP concentration in aqueous solution is calculated from absorbances at four wavelengths: the rationale is of general applicability to nucleosides and nucleotides.     

Intranasal administration of adjuvant-combined recombinant influenza virus HA vaccine protects mice from the lethal H5N1 virus infection

Attenuated recombinant H5N1 influenza virus was constructed to develop a safe H5N1 influenza vaccine. The immunogenicity and protective effect of the vaccine prepared from haemagglutinin-modified recombinant H5N1 influenza virus was evaluated in mice intranasally co-administered with cholera toxin B subunit containing a trace amount of holotoxin (CTB*), synthetic double-stranded RNA, poly (I:C) or chitin microparticles (CMP) as adjuvants. Intranasal administration of recombinant H5 HA split vaccine with CTB* or poly(I:C) and/or CMP elicited an immunological response with both anti-H5 HA IgA in the nasal wash and anti-H5 HA IgG antibody in the serum, and showed a protective against lethal H5N1 A/Hong Kong/483/97 (HK483) infection. We also demonstrated that intranasal co-administration of antigen with both poly (I:C) and CMP enhanced the expression of Toll-like receptor (TLR) 3, TLR7 in the spleen. These results indicate that poly (I:C) and CMP are highly effective as mucosal adjuvants for use with the nasal H5N1 vaccine.     

响应面法优化北豆根粗多糖的除蛋白工艺及其神经保护活性研究

为研究北豆根粗多糖的最佳除蛋白方法和工艺,探究北豆根粗多糖的神经保护活性。实验比较了酶法、Sevage法、酶-Sevage法、三氯乙酸(TCA)-正丁醇法、酶-TCA-正丁醇法除蛋白效果,筛选出了北豆根粗多糖的最佳除蛋白方法,并用响应面法对该方法进行优化。经响应面分析,以综合评分为指标,考查TCA与正丁醇体积比、北豆根粗多糖溶液与TCA-正丁醇溶液体积比和振摇时间对北豆根粗多糖TCA-正丁醇法除蛋白工艺的影响。用H_2O_2诱导PC12细胞损伤,探究了北豆根粗多糖的神经保护作用。结果表明,北豆根粗多糖的最佳除蛋白方法为TCA-正丁醇法。经响应面优化,确定最优除蛋白工艺为TCA:正丁醇=1∶10.4,北豆根粗多糖溶液:TCA-正丁醇溶液=1∶1.77,振摇时间为36.5 min。采用该工艺对北豆根多糖进行除蛋白,其蛋白清除率为73.1%,综合评分为92.1。神经保护研究结果表明,北豆根粗多糖对H_2O_2诱导的PC12细胞损伤具有明显的保护作用。本研究表明TCA-正丁醇法可以有效的除去北豆根粗多糖中的蛋白质且北豆根粗多糖具有神经保护活性。     

Detection of the cholera toxin-binding activity of kappa-casein macropeptide and optimization of its production by the response surface methodology

The cholera toxin (CT)-binding activity of purified kappa-casein macropeptide (CMP) from bovine kappa-casein was detected. In addition, a statistical model was developed to optimize the production of CMP. CMP was prepared by chymosin hydrolysis of kappa-casein and a subsequent 3% trichloroacetic acid treatment. CMP was further fractionated in an ion-exchange column by FPLC. CT binding activity was eluted at 0.18 M NaCl and was a single 8.9 kDa peptide without tyrosine and arginine residues. The CT binding activity was rapidly lost by a carbohydrase treatment. The conditions for CMP production with chymosin were optimized by using the response surface methodology (RSM). The estimated optimum levels of the factors were as follows: reaction temperature, 38.5 degrees C; pH, 6.44; and time, 35.9 min. A validation experiment was performed in which CMP was prepared under the predicted parameters, and it was ascertained that the estimated optimum conditions gave better production of CMP than any other conditions.     

白灵菇多糖对运动小鼠氧化应激的影响

体外研究表明,白灵菇多糖具有较高的清除自由基能力。然而,白灵菇多糖在体内对运动引起的氧化应激的影响尚不清楚。本研究将100只SPF级雄性昆明小鼠随机分为5组,低剂量组、中剂量组和高剂量组昆明小鼠分别按照50 mg·kg^-1·d^-1、100 mg·kg^-1·d^-1和200 mg·kg^-1·d^-1的剂量灌胃白灵菇多糖溶液,对照组和模型组昆明小鼠灌胃等体积的蒸馏水,连续灌胃4周。研究显示,白灵菇多糖溶液以浓度依赖性方式提高了小鼠的力竭游泳时间(p<0.05)。白灵菇多糖以浓度依赖性方式降低了小鼠血清AST、ALT和CK水平,并显著减少了骨骼肌的病理变化(p<0.05)。白灵菇多糖以剂量依赖方式升高力竭游泳小鼠体内SOD、CAT和GSH-PX水平,并降低了MDA水平(p<0.05)。此外,对小鼠灌胃白灵菇多糖可以剂量依赖方式提高小鼠血清总抗氧化活性(p<0.05)。上述研究表明,白灵菇多糖可有效提高力竭游泳小鼠的抗疲劳能力,减轻运动引起的心肌、肝脏、骨骼肌和氧化应激损伤,提高机体的抗氧化能力。     

Immunomodulatory and antioxidant effects of carboxymethylpachymaran on the mice infected with PCV2

The objective of the current study is to investigate the protective effect of carboxymethylpachymaran (CMP) on the immune system of mice via multiple infections with porcine circovirus type 2 (PCV2). The in vivo results showed that CMP administration significantly improved the spleen or thymus index, promoted the proliferation activities of T or B lymphocytes, and increased the production of glutathione, the superoxidase dismutase capacity, and the total antioxidant capacity in the spleen or thymus of PCV2-infected mice. The administration of different CMP doses to PVC2-inoculated mice resulted in the upregulation of IL-2 and IFN-α or the downregulation of IL-10 levels in the serum. These findings suggest that CMP has potential applications in regulating immunological functions to overcome the immunosuppresion caused by PCV2 infection in mice. The findings may also prove useful in designing effective therapies against PCV2 infection.