PEG修饰尿酸酶纯化方法的优化

[目的]探索一种聚乙二醇修饰尿酸酶后的纯化方法,提高分离纯化效率,保留酶的活性,适用性广,便于扩大生产.[方法]60％饱和度硫酸铵溶液初步纯化,阴离子柱层析,最后用分子排阻法精纯.[结果]初步纯化酶活达到110U,精纯之后,聚乙二醇修饰尿酸酶纯度可达100％,NHS和PEG残留被纯化分离,平均每个尿酸酶单体被10个PE...     

聚唾液酸与唾液酸的研究进展

唾液酸是一族神经氨酸(Neuraminic acid)的衍生物。聚唾液酸(Polysialic acid)是唾液酸(Sialic acid)单体以α-2,8或α-2,9键连接的直链同聚物,是一些哺乳动物细胞中糖蛋白的组成部分和少数几种细菌的胞外多糖组分。综述了唾液酸和聚唾液酸的结构、性质、生物学功能、生物合成和生产应用。     

聚唾液酸的发酵动力学研究

对以大肠杆菌K235发酵法生产聚唾液酸的动力学特性进行了研究,提出了细胞生长动力学,基质消耗动力学,聚唾液酸生成动力学模型,通过对实验数据的计算,模型的模拟结果较好地和实验值吻合,正确地分析 聚唾液酸的发酵过程及其动力学机制。     

聚唾液酸,一种非GAGs、非免疫原性生物材料的应用研究进展

聚唾液酸是一种由N-乙酰神经氨酸连接、电负性的线性同聚物,存在于人体、动物细胞和少数致病菌中,主要以糖蛋白(神经细胞粘附分子)和糖脂形式存在,是一种非糖胺聚糖(GAGs)、非免疫原性、生物可降解的优良生物材料。聚唾液酸可用作组织工程和药物缓释材料,也可以与其它大分子复合形成功能材料。对聚唾液酸生物学功能、发酵生产及应用进行概述,以期为聚唾液酸的进一步应用研究提供参考。     

端基法测定聚唾液酸平均聚合度

建立了端基法测定聚唾液酸平均聚合度的方法.采用间苯二酚比色法和丙二腈荧光法分别测定聚唾液酸中唾液酸总量和还原端唾液酸残基含量,两者之比即为平均聚合度.研究表明,在pH 9.5的硼酸缓冲液中,80℃水浴下聚唾液酸还原端唾液酸残基与丙二腈反应25 min后生成荧光物质,其荧光强度与还原端唾液酸残基含量呈线性正相关关系,线性范围在1～ 20 mg/L之间,变异系数和检出限分别为3.7％和0.36 mg/L.端基法测定大肠杆菌发酵液中聚唾液酸的平均聚合度为45.76,与高效液相凝胶色谱法比较,误差为3.2％.该法可以简便快速地测定发酵液中聚唾液酸的平均聚合度,有利于聚唾液酸生产过程分析及产品性能评估.     

两阶段搅拌转速控制策略发酵生产聚唾液酸

目的:优化聚唾液酸发酵过程的搅拌转速.方法:比较不同搅拌转速对大肠杆菌Escherichia coli K235分批发酵生产聚唾液酸过程的影响.结果:根据发酵前、后期菌体细胞比生长速率和聚唾液酸比合成速率达到最大值所需搅拌转速的不同,提出了两阶段搅拌转速控制策略:发酵前期(0～15h)控制搅拌转速500r/min,发酵中后期控制搅拌转速700r/min.结论:两阶段搅拌转速控制策略使聚唾液酸产量达到3 966mg/L,比恒定搅拌转速500r/min和700r/min分别提高了31.8%和49.3%.将两阶段搅拌转速控制策略与分批补料发酵技术结合,聚唾液酸产量提高到5 108mg/L,山梨醇的转化率达到0.12g/g.     

聚乙二醇修饰β-干扰素的研究

采用平均分子量为5kD的已活化的单甲氧基聚乙二醇(mPEG)对重组人β-干扰素(rhIFN-β)进行化学修饰。优化修饰条件,选择对rhIFN-β反应性高的修饰剂,制备三种不同修饰程度的修饰物,并对修饰物进行初步检定。三种修饰物的修饰率分别为10．12％、22．99％、42．47％;比活性分别保留为原来的93．53％、48．69％、13．18％;PEG修饰后的rhIFN-β在pH7时的溶解度增加。     

干扰素α-2b的聚乙二醇修饰

采用分子量为20 kD的单甲氧基聚乙二醇丙醛(mPEG-ALD)修饰重组人干扰素α-2b(IFN α-2b),建立了修饰反应及分离纯化工艺.考察了修饰反应各因素对单修饰转化率以及单修饰产物体外活性的影响,获得了优化的修饰反应条件,即在pH 6.5,20 mmol/L的磷酸氢二钠-柠檬酸缓冲溶液中,干扰素α-2b的浓度为4 mg/mE,PEG与IFN α-2b的摩尔比为8:1,4℃时反应20 h;在优化的反应条件下,单修饰PEG-IFN α-2b的转化率达到55%.并且,采用离子交换层析对修饰产物进行分离纯化,单修饰产品纯度达到97%,体外活性保留达到未修饰干扰素α-2b的13.4%,其在SD大鼠体内的循环半袁期得到了较大的延长,且具有较好的水溶液稳定性.     

蛋白质药物的聚乙二醇修饰

聚乙二醇被广泛应用于蛋白质药物的化学修饰,修饰后的蛋白质药物的性质发生多方面变化,如:增加了此类药物的溶解度和稳定性,耐酶水解的能力增强,减弱或消除免疫原性,增加药物在体内的半衰期等。近年来,聚乙二醇修饰剂的种类和修饰方法发展较快,蛋白质分子上的氨基、巯基、羧基均成为化学修饰的研究对象。本文综述了聚乙二醇修饰的原理与方法,修饰方法的比较与优化,修饰后产品的鉴定与检测。     

丙酮酸钠对E．coli CCTCCM208088发酵生产聚唾液酸的影响

研究了丙酮酸钠对E．coliCCTCCM208088发酵生产聚唾液酸的影响。首先在摇瓶水平上优化了丙酮酸钠的添加策略：发酵初始培养基中添加6g／L丙酮酸钠,聚唾液酸的产量达到最高水平3．47g／L,相比空白相比提高了73％,聚唾液酸产率（YP／（x．s））提高了125％。在30L发酵罐中,添加丙酮酸钠使聚唾液酸产量达到了6．6g／L,相对照提高了53．5％。通过有机酸分析,添加丙酮酸钠增强了菌体内三羧酸循环．可能导致胞内能荷水平的提高．从而促进了聚唾液酸的合成。     

Arginine-specific modification of proteins with polyethylene glycol

In this study, the residue-selective modification of proteins with polymers at arginine residues is reported. The difficulty in modifying arginine residues lies in the fact that they are less reactive than lysine residues. Consequently, typical chemo-selective reactions which employ "kinetic" selectivity (active esters, Michael addition, etc.) cannot be used to target these residues. The chemistry exploited herein relies on "thermodynamic" selectivity to achieve selective modification of arginine residues. ω-Methoxy poly(ethylene glycol) bearing an α-oxo-aldehyde group was synthesized and used to demonstrate the selective modification of lysozyme at arginine residues. In addition, the optimization of reaction conditions for coupling as well as the stability of the formed adduct toward dilution, toward a nucleophilic buffer, and toward acidification are reported. It was concluded that this approach is a convenient, mild, selective, and catalyst-free method for protein modification.     

Chemical modification of Vibrio vulnificus metalloprotease with activated polyethylene glycol

Abstract Vibrio vulnificus , an opportunistic human pathogen causing septicemia, produces a metalloprotease which is suspected to be a virulence determinant, but which is labile in vivo due to inactivation by α -macroglobulin. To obtain a derivative which is stable in vivo, the metalloprotease was modified with activated monomethoxy polyethylene glycol. The modified protease retained full activity to a peptide substrate and 10–20% activity to protein substrates, and was resistant to entrapment by α -macroglobulin because of the increased molecular size (approx. 90 kDa). These findings suggest that the modified protease is stable in vivo and may be used to investigate the pathological actions of the protease in the bloodstream.     

Improvement of proteolytic resistance of immunoadsorbents by chemical modification with polyethylene glycol

Immunoadsorbents were modified with monomethoxy-polyethylene glycol (PEG; average molecular weights of 5000 (PEG-5000) and 1900 (PEG-1900)) activated with cyanuric acid (activated PEG) by four different methods. In the two methods, anti-BSA antibodies were modified with activated PEG with and without protection of antigen binding sites with BSA and then were coupled to CNBr-activated Sepharose 4B. In the other two methods, Immunoadsorbents, which were prepared by coupling anti-BSA antibodies to CNBr-activated Sepharose 4B, were modified with activated PEG with and without the protection. The effects of PEG modification by these four methods on the binding ratio (the ratio of the numbers of moles of antigen adsorbed to the numbers of moles of binding sites of antibody coupled), the antigen binding property and the resistance to proteolytic digestion of immunoadsorbents were studied. The decrease in the binding ratio by the modification with activated PEG was small enough to use modified immunoadsorbents for industrial purification processes. The resistance to proteolytic digestion of immunoadsorbents was improved by modification with activated PEG. The modification without protection of antigen binding sites gave higher resistance to proteolytic digestion than that with protection, while the former caused larger decrease in the binding ratio of modification. The immunoadsorbents modified with activated PEG-5000 showed higher resistance to proteolytic digestion than those modified with activated PEG-1900.     

重组L-门冬酰胺酶工程菌的表达和PEG的化学修饰

目的提高重组L-门冬酰胺酶(rL-ASP)工程菌的表达量,分离纯化rL-ASP并对之进行PEG化学修饰。方法将带有编码rL-ASP的基因的质粒(pKA)导入不同的宿主菌中,挑出高表达菌株,同时优化发酵培养基,分离纯化获得的高纯度rL-ASP再用PEG进行化学修饰,SDS-PAGE检测修饰效果。结果在pH7.0的条件下,宿主菌为JMl09的工程菌pKA/JMl09酶活力最高,三角瓶振摇培养的酶活力可达216×103IU/L;发酵罐发酵培养,酶活力达312×103IU/L。纯化后的rL-ASP比活力为220IU/mg,rL-ASP经过PEG化学修饰生成rL-ASP-PEG,分子量发生改变。结论改变目标蛋白表达的宿主菌和优化发酵工艺,提高了rL-ASP的表达量,纯化的rL-ASP经过PEG化学修饰后分子量增大。     

New PEG2 type polyethylene glycol derivatives for protein modification

Although proteins with 2,4-bis (o-methoxypolyethylene glycol)-6-chloro-s-triazine (PEG2-Cl) as a divalent PEG modification have some advantages compared to proteins with the linear PEG modification, PEG2Cl cannot react with amino groups at neutral pH. Therefore, we have prepared new PEG2 derivatives that have an activated ester as the functional group. We confirmed that these derivatives are useful for the divalent modification of proteins, such as bSOD and rhG-CSF. © Rapid Science Ltd. 1998     

Chemical modification of L-asparaginase with a comb-shaped copolymer of polyethylene glycol derivative and maleic anhydride.

L-Asparaginase from Escherichia coli, an anti-tumor enzyme, was chemically modified with two types of maleic anhydride copolymers with a comb-shaped form, the one composed of polyoxyethylene allyl methyl diether with the molecular weight of 13,000 (activated PM13) and the other of polyoxyethylene 2-methyl-2-propenyl methyl diether with 100,000 (activated PM100). The modified asparaginases (PM13- and PM100-asparaginases) exhibited the complete loss of immunoreactivity towards anti-asparaginase serum. The enzymic activity of PM100-asparaginase without immunoreactivity was well retained by 85% of non-modified one, while that of PM13-asparaginase was retained 46%. These results were discussed in relation to the chemical structure of modifying reagents including chain shaped-polyethylene glycol derivatives.     

Improved germination in seeds of guayule (Parthenium argentatum Gray) following polyethylene glycol and gibberellic acid pretreatments

Suitable conditions for the pretreatment of seeds of guayule were determined with a view to improving germination. These included the addition of thiram (500 mg litre^-1), and applications of GA₄₊₇ alone, or in combination with polyethylene glycol. Significant improvements in the seed germination were seen following applications of PEG at -0.10 MPa. Simultaneous application of GA₄₊₇ with priming improved soil emergence and germination over a wide range of temperatures. No beneficial effects of PEG priming were evident on seed storage.     

新一代PEG在修饰抗原和药物缓释中的应用

聚乙二醇及其衍生物是具有许多优良性质的高分子化合物,由于良好的生物相容性、无毒、无免疫原性,广泛用于生物医学领域。本文总结聚乙二醇的发展历史和新一代聚乙二醇的特点,阐述聚乙二醇化修饰的目的,特别是在抗原修饰、血型改造和细胞移植等方面的应用,重点对聚乙二醇在药物缓释方面的应用进行了系统的综述。     

Acceleration of nucleic acid hybridization rate by polyethylene glycol

The addition of polyethylene glycol to filter-bound nucleic acid hybridization greatly increases the hybridization rate. With single-stranded probes, the increase obtained with polyethylene glycol is significantly greater than that obtained with dextran sulfate. Additionally, polyethylene glycol is easier to manipulate and less expensive than dextran sulfate.