对分离在不同营养培养基上的复合脓肿分枝杆菌菌株质谱的比较分析

IF 1.6 Q4 INFECTIOUS DISEASES International Journal of Mycobacteriology Pub Date : 2024-07-01 Epub Date: 2024-09-14 DOI:10.4103/ijmy.ijmy_135_24
Ekaterina Vasilievna Vyzhigina, Alexander Mikhailovich Kovalyov, Daniil Andreevich Kokorev, Elena Alexandrovna Borodulina, Danir Damirovich Ismatullin, Artem Viktorovich Lyamin
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引用次数: 0

摘要

背景:复合脓肿分枝杆菌(MABSc)会导致患者慢性感染,同时伴有呼吸道结构的改变,这对囊性纤维化患者尤为重要。要从临床材料中分离出 MABSc 培养物,需要使用各种营养培养基。要确定在这些培养基上分离出的微生物的种类,还需要使用其他鉴定方法,如聚合酶链反应、测序或质谱法。后一种方法相对容易实施,但需要改进,因为非结核分枝杆菌的鉴定一般都不准确。因此,一套营养培养基可能对随后的质谱鉴定非常重要:研究对象为 64 株 MABSc 代表菌株:方法:研究对象为 64 株 MABSc 代表菌株:56 株来自囊性纤维化患者,8 株来自与囊性纤维化无关的肺部病变患者。将获得的 MABSc 菌株移植到通用发色培养基和选择性培养基中,用于分离伯克霍尔德氏菌复合体(BCC)。通过基质激活激光飞行时间解吸/电离(MALDI-ToF MS)质谱法进行菌种鉴定。微生物鉴定的依据是将获得的质谱与数据库中的参考质谱进行比较。微生物的鉴定基于重合度(得分值)。质谱鉴定微生物的样品制备采用扩展直接应用法。长度分别为 752 bp 和 441 bp 的 rpoB 和 hsp65 基因片段被用作分子标记,用于 MABSc 菌株的亚特异性鉴定:对在所研究的营养培养基上分离的 MABSc 菌株进行质谱分析后得到的峰值进行比较,结果表明这些指标与添加多聚麦芽糖氢氧化铁(III)的 BCC 分离选择性培养基和通用发色培养基(P < 0.001)以及添加通用发色培养基的 BCC 分离选择性培养基(P < 0.001)之间存在显著差异。对 25 株 MABSc 代表菌株进行了测序:在通用致色培养基上分离的菌株的亚种测定结果与 15 株菌株中 13 株(86.6%)的测序结果一致:MALDI-ToF 质谱法可在短时间内以最低成本鉴定微生物,但还不能正确鉴定某些微生物群(如 MABSc)的亚种。培养方法需要优化,细菌蛋白质部分的提取过程也需要新方法。
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Comparative Analysis of the Mass Spectra of Mycobacterium abscessus Complex Strains Isolated on Various Nutrient Media.

Background: Mycobacterium abscessus complex (MABSc) causes chronic infection in patients with concomitant structural changes in the respiratory tract, which is especially important for patients with cystic fibrosis. To isolate an MABSc culture from clinical material, a variety of nutrient media are used. For species determination of microorganisms isolated on these media, additional identification methods are used, for example, polymerase chain reaction, sequencing, or mass spectrometry. The latter method is relatively easy to implement but requires improvement, due to the identification inaccuracy of nontuberculosis mycobacterias in general. Consequently, a set of nutrient media may be important for subsequent identification by mass spectrometry.

Methods: The study was conducted on 64 strains of MABSc representatives: 56 strains were obtained from patients with cystic fibrosis and 8 strains from patients with pulmonary pathology unrelated to cystic fibrosis. The obtained MABSc strains were transplanted to the universal chromogenic medium and the selective medium for the Burkholderia cepacia complex (BCC) isolation. Species identification was carried out by mass spectrometry based on matrix-activated laser time-of-flight desorption/ionization (MALDI-ToF MS). Microbial identification is based on a comparison of the obtained mass spectra with reference spectra from the database. Microorganisms were identified based on the coincidence degree (Score value). Sample preparation for microbial identification by mass spectrometry was carried out by an extended direct application method. Fragments of the rpoB and hsp65 genes with lengths of 752 bp and 441 bp, respectively, were used as molecular markers for subspecific identification of MABSc strains.

Results: A comparison of the peaks obtained after mass spectrometry of MABSc strains isolated on the studied nutrient media showed significant differences between these indicators selective medium for the BCC isolation with the supplement of iron polymaltose hydroxide (III) and universal chromogenic medium (P < 0.001) and selective medium for the BCC isolation with universal chromogenic medium (P < 0.001). Twenty-five strains of MABSc representatives were sequenced: results of subspecies determination in strains isolated on the universal chromogenic medium coincided with the results sequencing in 13 (86.6%) strains out of 15.

Conclusion: MALDI-ToF mass spectrometry allows microbial identification in a short time and with minimal cost, but it does not yet allow the proper identification of the subspecies of certain microbial groups, such as MABSc. Cultivation methods need optimization and new approaches to the extraction process of the bacterial protein fraction.

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