McLAUCHLIN J, Mithani V, Bolton F J, Nichols G L, Bellis M A, Syed Q, Thomson R P M, Ashton J R
PHLS Food Safety Microbiology Laboratory, Central Public Health Laboratory and *Environmental Surveillance Unit, Communicable Disease Surveillance Centre, 61 Colindale Ave, London NW9 5HT, †Birkenhead & Wallasey Primary Care Trust, St Catherine's Hospital, Birkenhead, Merseyside CH42 0LP, ‡Communicable Disease Surveillance Centre (North West), Chester CH1 4EF, §South Sefton Primary Care Trust, Burlington House, Crosby Road North, Waterloo, Liverpool L22 0QB and ||Department of Public Health North West Region, Millennium Park, Birchwood, Warrington WA3 7QN.
J Med Microbiol. 2002 Nov;51(11):1001-1008. doi: 10.1099/0022-1317-51-11-1001.
In 2000, an unusual increase of morbidity and mortality among illegal injecting drug users in the UK and Ireland was reported and Clostridium novyi was identified as the likely source of the serious infection, although infections due to C. botulinum and Bacillus cereus were also reported. Because heroin was a possibile source of infection, this study investigated the microflora of heroin samples seized in England during 2000 and 2002. Two methods were developed for the examination of the microflora of heroin. The first consisted of suspension of the drug in maximum recovery diluent (MRD) which was inoculated directly into Clostridium Botulinum Isolation Cooked Meat Broth (CBI). The second method rendered the heroin soluble in citric acid, concentrated particulate material (and bacterial cells) by filtration and removed heroin residues by washing with citric acid and phosphate-buffered saline before placing the filter in CBI broth. Duplicate CBI broths from both methods were incubated without heating and after heating at 60 degrees C for 30 min. Subcultures were made after incubation for 7 and 14 days on to eight different solid media. The methods were evaluated with heroin samples spiked with either C. botulinum or C. novyi spore suspensions; recovery of 10 spores in the original sample was demonstrated. Fifty-eight heroin samples were tested by citric acid solubilisation and 34 by the MRD suspension technique. Fifteen different gram-positive species of four genera were recognised. No fungi were isolated. Aerobic endospore-forming bacteria (Bacillus spp. and Paenibacillus macerans) were the predominant microflora isolated and at least one species was isolated from each sample. B. cereus was the most common species and was isolated from 95% of all samples, with B. licheniformis isolated from 40%. Between one and five samples yielded cultures of B. coagulans, B. laterosporus, B. pumilus, B. subtilis and P. macerans. Staphylococcus spp. were isolated from 23 (40%) samples; S. warneri and S. epidermidis were the most common and were cultured from 13 (22%) and 6 (10%) samples respectively. One or two samples yielded cultures of S. aureus, S. capitis and S. haemolyticus. The remainder of the flora detected comprised two samples contaminated with C. perfringens and two samples with either C. sordellii or C. tertium. Multiple bacterial species were isolated from 43 (74%) samples, a single species from the remaining 15. In 13 samples B. cereus alone was isolated, in one B. subtilis alone and in one sample B. pumilus alone. C. botulinum and C. novyi were not isolated from any of the heroin samples. Recommendations for the optimal examination of the microflora of heroin are given.
2000年,英国和爱尔兰报告称非法注射吸毒者的发病率和死亡率异常上升,诺维氏梭菌被确定为严重感染的可能来源,不过也有肉毒杆菌和蜡样芽孢杆菌感染的报告。由于海洛因可能是感染源,本研究调查了2000年和2002年在英格兰查获的海洛因样本的微生物群落。开发了两种检测海洛因微生物群落的方法。第一种方法是将药物悬浮在最大回收稀释液(MRD)中,然后直接接种到肉毒杆菌分离熟肉培养基(CBI)中。第二种方法是使海洛因可溶于柠檬酸,通过过滤浓缩颗粒物质(和细菌细胞),并用柠檬酸和磷酸盐缓冲盐水洗涤以去除海洛因残留,然后将过滤器放入CBI肉汤中。两种方法的一式两份CBI肉汤在不加热以及在60℃加热30分钟后进行培养。培养7天和14天后,将培养物接种到八种不同的固体培养基上进行传代培养。用接种了肉毒杆菌或诺维氏梭菌孢子悬液的海洛因样本对这些方法进行评估;结果表明在原始样本中可回收10个孢子。通过柠檬酸溶解法检测了58个海洛因样本,通过MRD悬浮技术检测了34个样本。识别出四个属的15种不同的革兰氏阳性菌。未分离出真菌。需氧芽孢杆菌(芽孢杆菌属和浸麻芽孢杆菌)是分离出的主要微生物群落,每个样本至少分离出一个菌种。蜡样芽孢杆菌是最常见的菌种,从所有样本的95%中分离得到,地衣芽孢杆菌从40%的样本中分离得到。有1至5个样本培养出凝结芽孢杆菌、侧孢芽孢杆菌、短小芽孢杆菌、枯草芽孢杆菌和浸麻芽孢杆菌。从23个(40%)样本中分离出葡萄球菌属;华纳葡萄球菌和表皮葡萄球菌最常见,分别从13个(22%)和6个(10%)样本中培养得到。有1或2个样本培养出金黄色葡萄球菌、头葡萄球菌和溶血葡萄球菌。检测到的其余菌群包括2个被产气荚膜梭菌污染的样本以及2个被索氏梭菌或第三梭菌污染的样本。43个(74%)样本分离出多种细菌,其余15个样本分离出单一菌种。13个样本仅分离出蜡样芽孢杆菌,1个样本仅分离出枯草芽孢杆菌,1个样本仅分离出短小芽孢杆菌。未从任何海洛因样本中分离出肉毒杆菌和诺维氏梭菌。文中给出了海洛因微生物群落最佳检测方法的建议。
