磁性聚合物微球固定化青霉素G酰化酶制备光学纯(S)-2-氯苯甘氨酸

通过反相悬浮聚合法制备了超顺磁性环氧聚合物微球用于固定化青霉素G酰化酶,利用磁性固定化酶催化N-苯乙酰-(R,S)-2-氯苯甘氨酸进行不对称水解反应,制备出(S)-2-氯苯甘氨酸单一对映体。磁性固定化酶催化水解反应的适宜条件为:底物浓度100 mg·m L-1,反应温度和时间30℃和12 h,反应溶液p H 8.0。在此条件下,N-苯乙酰-(R,S)-2-氯苯甘氨酸的转化率为48.8%,产物(S)-2-氯苯甘氨酸的对映体过量值eep达99.4%。磁场下回收磁性固定化青霉素G酰化酶,重复使用6次,底物的转化率和产物的对映体过量值分别为47.8%和91.4%。     

Organically modified xerogels as novel tailor-made supports for covalent immobilisation of enzymes (penicillin G acylase)

A novel application of organically modified silicates for covalent immobilisation of penicillin G acylase is reported. The immobilisation is efficient and the enzymatic preparation shows high specific activity and thermal stability. The technique opens new perspectives for the preparation of innovative tailor-made supports matching specific requirements of enzymatic processes.     

酶法拆分D,L-苯丙氨酸制备D-苯丙氨酸

在固定化青霉素酰化酶(IPA-750)存在下,通过N-苯乙酰-D,L-苯丙氨酸(2)的选择性水解完成了酶法拆分D,L-苯丙氨酸(1)制备D-苯丙氨酸(5)的过程。选择性水解的较适宜反应条件为:22.83g,m(2)∶m(IPA-750)=6∶1,pH7.0,于30℃反应5h,产物为N-苯乙酰-D-苯丙氨酸(4)和L-苯丙氨酸(3,收率63%,光学纯度99%)。4用6mol·L-1盐酸于120℃水解反应8h,经脱盐处理得5,收率67%,光学纯度91%。3在含醋酸酐的醋酸溶液中进行消旋化处理,得到100%消旋的1可继续进行下一轮酶法拆分。     

青霉素钾对微乳液增溶作用的影响

层状液晶;青霉素钾对微乳液增溶作用的影响     

青霉素 V钾的二次微分简易示波伏安法测定

利用青霉素 V钾在 pH=7的 KH2PO4-Na2HPO4缓冲溶液中产生切口的示波特性 , 提出了一种药片中青霉素 V钾的测定方法 - - 二次微分简易示波伏安法 ; 校正曲线的线性范围为 2.0× 10-5～ 2.0× 10-4 mol/L, 检出限为 8× 10-6 mol/L; 对 7.0× 10-5 mol/L青霉素 V钾 8次测定结果的相对标准偏差为 1.6% ; 实验结果表明该法具有分析速度快、仪器装置简单以及药片中的淀粉等物质不干扰测定的优点 .     

Immobilization of penicillin acylase in porous beads of polyacrylamide gel

A procedure is described for the immobilization of benzylpenicillin acylase from Escherichia coli within uniformly spherical, porous polyacrylamide gel beads. Aqueous solutions of the enzyme and sodium alginate and of acrylamide monomer, N,N'-methylene-bis-acrylamide, N,N,N,N'-tetramethylethylenediamine (TEMED) and sodium alginate are cooled separately, mixed, and dropped immediately into ice-cold, buffered calcium formate solution, pH 8.5, to give calcium alginate-coated beads. The beads are left for 30-60 min in the cold calcium formate solution for polyacrylamide gel formation. The beads are then treated with a solution of glutaraldehyde and the calcium alginate subsequently leached out with a solution of potassium phosphate. Modification of the native enzyme with glutaraldehyde results in a slight enhancement in the rate of hydrolysis of benzylpenicillin at pH 7.8 and 0.05M substrate concentration. The enzyme entrapped in porous polyacrylamide gel beads shows no measurable diffusional limitation in stirred reactors, catalyzing the hydrolysis of the substrate at a rate comparable to that of the glutaraldehyde-modified native enzyme. The immobilized enzyme preparation has been used in batch mode over 90 cycles without any apparent loss in hydrolytic activity.     

Determination of Penicillins in Milk by a Dual-Optrode Biosensor

Penicillins are the most frequently found antibiotic residues in milk, as they are commonly used for the treatment of bacterial infections in cows. In the present study, we introduce a method for the rapid detection of penicillin residues in raw milk based on the determination of glucose concentration in milk with a dual flow-through biosensor. The molar concentration of glucose in milk is typically over 500 times lower than the concentration of lactose and is highly dependent on the rate of lactose hydrolysis, which is catalyzed by β-galactosidase. Glucose concentrations in milk change with variation in the β-galactosidase activity. β-Galactosidase is an enzyme produced in the microbiota in milk and its activity is inhibited by benzylpenicillin. Spiking milk with benzylpenicillin lowers glucose concentrations in comparison to high-quality milk after short storage intervals. The presence of penicillin in the milk of treated animals resulted in decreased glucose concentrations in comparison with high-quality milk that contained no antibiotics. The glucose concentration in milk samples was followed by the system enabling the elimination of the effects of bacterial respiration in the output with reliable results in less than 1?min.     

A Facile and Highly Stereoselective Reductive Dcbromination of AnhydrO-6- (R)-Hydroxyethyl- 6-Bromopenicillin

Thetitlecompound,4-acetoxyazetidinone5',hasbeenwidelyusedasanimportantintermediateforpenem,carbapenemandtrinemsynthesisZa~Zfandseveralapproachesto5havebeenreported3a~3c.Thesemisyntheticapproachof4-acetoxyazetidinone5frompenicillinIreportedbyDiNinnoetal.Zbisausefulone,thedebrominationofmethyl6-bromo-6-l(R)-Ihydroxy-ethyllpenicillinate3byzinc-ammoniumacetateaffordedthelabilecompound4.91igmixtureoftransandetsisomers,in92%yieldbutintheformerstepthehydroxyethylationoftheC-6positionofpenicillinat…     

Application of spontaneous suction phase-dispersing (SSPD) extractors in the extraction of penicillin G

The extraction of penicillin G from an aqueous solution with butylacetate (BA) and tributyl phosphate (TBP) as extractants was carried out at pH 4 with spontaneous suction phase-dispersing (SSPD) extractors under various operating conditions. Four kinds of SSPD extractors were tested with results compared to those obtained by using an extractor with mechanical stirrers. Rotation speed and different extraction systems were found to influence the penicillin recovery and the stability of emulsion formed during extraction. The percentage of extraction under optimum conditions was 91% without formation of emulsion. The laser particle size measurement instrument combined with SSPD can be used to measure the emulsion droplet size in situ.     

Development of quantitative HPTLC-densitometry methods following a model approach for transfer of TLC screening methods for pharmaceutical products of atenolol,chloramphenicol, furosemide,glibenclamide, penicillin V potassium,and praziquantel

Transfer of six thin-layer chromatography (TLC) Global Pharma Health Fund E.V. Minilab manual protocols for detecting fake drugs in pharmaceutical products to quantitative high-performance TLC (HPTLC)-densitometry methods was performed following a previously published model process. The developed and validated methods for tablets or capsules containing atenolol, chloramphenicol, furosemide, glibenclamide, penicillin V potassium, and praziquantel involved use of a limited list of inexpensive, relatively nontoxic, readily available solvents and other reagents; silica gel 60?F₂₅₄ plates; automated bandwise sample and standard solution application; ascending mobile phase development of plates in a chamber; and automated slit scanning densitometry for detection, identification, and quantification. Validation data for methods developed in an early version of the transfer model process that did not include standard addition validation are reported for pharmaceutical products containing amitriptyline HCl, amodiaquine, diphenhydramine HCl, and mebendazole.