重组人戊型肝炎疫苗细菌内毒素检查方法的建立

确立重组人戊型肝炎疫苗原液的细菌内毒素检查方法。供试品参照《中华人民共和国药典》(2005年版三部)热原检查法进行热原检查,结果符合规定。该供试品同时参照《中华人民共和国药典》(2005年版三部)细菌内毒素检查法要求进行试验。供试品溶液在40μg/m l浓度下,确定内毒素限值为40EU/m l。供试品在该内毒素限值下干扰试验有效,且细菌内毒素检查法符合规定。该疫苗用内毒素检查法代替热原检查法,方法可行。     

刺五加注射液的细菌内毒素检查探讨

细菌内毒素检查法与热原检查法相比 ,成本低、快速简便、灵敏度高。为探讨采用细菌内毒素检查法检测刺五加注射液热原的可行性 ,我们进行了鲎试剂灵敏度复核试验、干扰试验 ,结果表明刺五加注射液稀释 2 .85倍 ,用灵敏度为 0 .2 5 EU·ml-1的鲎试剂作细菌内毒素检查 ,仍有干扰。1　实验材料　　鲎试剂 (批号 0 30 4 1 9,标示灵敏度 0 .5 EU·ml-1;批号 0 30 5 0 3,标示灵敏度 0 .2 5 EU· ml-1,福州新北生化工业有限公司 ) ;细菌内毒素工作标准品 (批号 2 0 0 30 3,规格 1 5 0 EU·支 -1,中国药品生物制品检定所 ) ;鲎试剂溶解水 (批号 …     

苦碟子注射液细菌内毒素检查法的探讨

目的：建立苦碟子注射液静脉点滴用药时细菌内毒素的检查方法。方法：采用2个厂家的鲎试剂对苦碟子注射液进行干扰试验。结果：鲎试剂浓度为0．25EU／mL时,苦碟子注射液稀释至1／30对细菌内毒素测定无干扰。结论：鲎试剂法检测苦碟子注射液静脉点滴用药时的细菌内毒素是可行的。     

静注人免疫球蛋白细菌内毒素检查方法的建立

目的 :建立用于静脉注射用人免疫球蛋白 (IVIG)的细菌内毒素检查方法。方法 :通过干扰评价实验证明IVIG对细菌内毒素检查法有强烈的抑制作用 ,单纯用简单稀释和调整pH值法无法消除干扰 ,如果用稀释剂 (Ⅰ )对IVIG作 1∶4以上的稀释 ,即可消除样品对该检查法的干扰 ,利用灵敏度为 0 1 2 5EU ml的鲎试剂 ,将样品用稀释剂 (Ⅰ )稀释 4倍 ,按中国药典 ( 2 0 0 0版 )进行细菌内毒素的检查 ,结果与家兔热原质试验进行比较。结论 :IVIG用稀释剂 (Ⅰ )进行适当稀释后 ,可以用细菌内毒素检查法替代家兔热原试验 ,应用于生产过程及半成品的质量控制。     

四种氨基酸原料细菌内毒素检查法的研究

依据中国药典2000年版“细菌内毒素检查法”,通过鲎试剂的干扰试验,研究注射用氨基酸原料中细菌内毒素检查法的可行性。结果在2~16倍稀释级下,L-缬氨酸(c=2.5%)和L-异亮氨酸(c=2.5%)对鲎试剂无干扰,检测细菌内毒素的鲎试剂灵敏度≤5.0×102EU.L-1,而在16倍稀释级范围内,L-脯氨酸(c=4.5%)和L-亮氨酸(c=2.0%)对鲎试剂检查法有抑制作用。结论为注射用L-异亮氨酸和L-缬氨酸用灵敏度为5.0×102EU.L-1的鲎试剂检查其细菌内毒素方法可行,可以代替家兔法检查热原。     

18-氨基酸注射液的动态浊度法检测研究

建立 18 -氨基酸注射液细菌内毒素定量测定方法 ,控制药品质量。采用动态浊度法 ,对 18-氨基酸注射稀释液进行干扰预实验、干扰实验定量检测。结果 18-氨基酸注射液在 8倍稀释时无干扰作用。因此用动态浊度法定量检查 18-氨基酸注射液细菌内毒素的含量 ,结果准确 ,在实际应用中完全可行。     

静脉注射用人免疫球蛋白细菌内毒素检测

探索静脉注射用人免疫球蛋白(IVIG)细菌内毒素含量的鲎试验检测方法。根据《中国药典》(2000版)细菌内毒素含量的检测方法进行,将待检品用NaOH调pH至中性,稀释至2.4倍可用标示灵敏度为0.25EU/m l的特异性鲎试剂进行细菌内毒素检测,结果与家兔法进行比较,并且在样品中加入定量内毒素0.6 EU/m l用两种方法进行对比试验。结果表明用细菌内毒素检测法(鲎试验法)检测静脉注射用人免疫球蛋白是可行的。     

用动态浊度法定量测定高聚生注射液中细菌内毒素

目的：探讨采用鲎试剂法对高聚生注射液进行细菌内毒素检查的可行性。方法通过试验确定高聚生注射液细菌内毒素检查的最大有效稀释倍数。结果：经干扰试验表明,内毒素的回收率在50％－200％之间。结论：高聚生注射液经最大有效稀释后进行细菌内毒素检查是可行的。     

浙江省热原检查用兔敏感性状况调查

目的调查浙江省热原检查用兔对细菌内毒素的敏感性情况,为提高热原检查结果的准确性和可靠性提供参考。方法对全省所有取得生产许可证单位的家兔,用国家颁发的细菌内毒素标准品,＂热原检查法＂进行检查,剂量分别为5EU/Kg和10EU/Kg,记录并比较各单位家兔的平均升温值和升温率。结果对细菌内毒素,各兔场家兔的敏感性有一定的差异。静脉注射5EU/kg,平均升温值为0.40℃～0.87℃,升温率为35%～83%;静脉注射10EU/kg,平均升温值为0.74℃～1.16℃,升温率为70%～94%。结论不同生产单位的家兔对细菌内毒素的敏感性不同,有必要对热原检查用家兔进行细菌内毒素敏感性检查。     

乙型脑炎灭活疫苗细菌内毒素检查方法的研究

将细菌内毒素检查法(凝胶法)扩大应用于乙脑灭活疫苗的质量控制及其内毒素的检测.按<中国药典>及<中国生物制品规程方法>方法,复核鲎试剂灵敏度、确定疫苗的L值、计算MVD、进行干扰试验及内毒素的检测.疫苗L值确定为300 EU/mL,MVD为1 200倍.用灵敏度0.25 EU/mL的鲎试剂,疫苗的最大非干扰浓度为将其稀释30倍,将此疫苗稀释120倍进行干扰试验,对内毒素的检测无干扰作用.以此法对15批疫苗进行内毒素检查均呈阴性反应.结果显示,此法用于乙脑灭活疫苗质量控制及其内毒素检查是可行的.     

Studies on the sensitivity and specificity of the Limulus amebocyte lysate test and rabbit pyrogen assays.

The sensitivity and specificity of the Limulus amebocyte lysate test and rabbit pyrogen assay were studied by means of artificially contaminated parenterals. Various gram-negative and gram-positive bacterial strains were used as was one strain of the yeast Candida albicans. The numbers of organisms needed to elicit positive responses in distilled water and normal saline were recorded and compared. The sensitivity and specificity of the Limulus amebocyte lysate assay for the detection of bacterial endotoxin from gram-negative bacteria were demonstrated. Variable results were recorded with gram-positive bacteria and Candida albicans.     

Studies on the sensitivity and specificity of the Limulus amebocyte lysate test and rabbit pyrogen assays

The sensitivity and specificity of the Limulus amebocyte lysate test and rabbit pyrogen assay were studied by means of artificially contaminated parenterals. Various gram-negative and gram-positive bacterial strains were used as was one strain of the yeast Candida albicans. The numbers of organisms needed to elicit positive responses in distilled water and normal saline were recorded and compared. The sensitivity and specificity of the Limulus amebocyte lysate assay for the detection of bacterial endotoxin from gram-negative bacteria were demonstrated. Variable results were recorded with gram-positive bacteria and Candida albicans.     

显色基质鲎试剂法在人血白蛋白热原检测中的应用

为了对显色基质法测定人血白蛋白中的内毒素含量方法进行探讨。以内毒素,鲎试剂及显色基质,在一定的条件下反应释放出对硝基苯胺(PNA),溶液呈现黄色,于波长545nm处比色读数,其产色深浅与内毒素浓度呈线性关系,从而定量测定出检品中内毒素含量。结果表明标准曲线的线性相关系数r≥0.98,人血白蛋白经3.3倍稀释后无干扰作用。显色基质法与家兔法比较,有灵敏、快速、能定量、重复性好的特点,可用于人血白蛋白内毒素含量的测定。     

Endotoxins in commercial vaccines.

Twenty samples of commercial vaccines intended for administration to humans were assayed for the presence of bacterial endotoxins by using the Limulus amebocyte lysate test. Sixteen of the vaccines contained more than 0.1 ng of endotoxin per ml (which corresponds to 103 bacterial cell wall equivalents per ml in the undiluted vaccines). These results suggest that at some stage of preparation, the vaccines have contained varying amounts of gram-negative bacteria and may indicate the presence of other bacterial products as well. It might be useful to list the level of endotoxins, phage, and other contaminants on each vaccine lot to facilitate studies on any side effects of these contaminants. Selection of vaccine lots with the least endotoxin might reduce some of the adverse effects of vaccinations.     

Early detection of the Limulus amebocyte lysate reaction evoked by endotoxins

The gelation of Limulus amebocyte lysate (LAL) evoked by bacterial endotoxins can be detected earlier than with usual methods by using laser scattering photometry to recognize the formation of small particles of clotted enzyme produced when the reaction mixture is agitated. The appearance of these small particles means that the influence of endotoxins has stimulated activation of the clotting enzyme across the LAL cascade, and the timing of their appearance is related to endotoxin concentration. This new method can be used for quick and sensitive endotoxin assay. The average endotoxin level of healthy volunteers was assayed to be 0.0738 pg/ml [0.0312-0.3445 pg/ml] (n = 11) within 70 min from the start of the assay.     

3种革兰氏阴性细菌及其L型内毒素含量的测定

本文采用鲎试剂对大肠杆菌（ＡＴＣＣ２５９２２）、伤寒杆菌、绿脓杆菌（ＡＴＣＣ７８５３）及它们的Ｌ型内毒素的含量进行测定。结果显示细菌型与细菌Ｌ型均具有内毒素,但细菌Ｌ型内毒素含量较细菌型低（约为１／３￣１／２）。因此,认为细菌Ｌ型仍有一定的致病性。     

Endotoxin detection and elimination in biotechnology

Endotoxins liberated by gram-negative bacteria are frequent contaminants of aqueous and physiological solutions. Because of their potent biological effects in vivo and in vitro, their detection and removal are essential for the safe parenteral administration of products produced from natural sources, as well as those produced by recombinant DNA technology. Traditional methods of endotoxin detection include the U.S. Pharmacopeia rabbit test and the Limulus amebocyte lysate test. Elimination of endotoxins, however, continues to be a problem. Standard methods of sterilization, such as autoclaving or sterile filtration, have little effect on endotoxin levels. Various techniques for the prevention of endotoxin contamination and endotoxin removal have been discussed. The overall role of endotoxin prevention, detection, and elimination in biotechnology is emphasized.