李斯特菌积累菌群的营养培养基设计

N. M. Khaptanova, S. V. Lukyanova, V. I. Kuznetsov, N. G. Gefan, N. M. Аndreevskaya, Z. A. Konovalova, А. S. Ostyak, V. S. Kosilko
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引用次数: 0

摘要

背景。为了获得鉴定李斯特菌的可靠的实验室研究结果,需要有经过认证的诊断凝集李斯特菌血清。在制造这种体外诊断医疗设备的过程中,一个重要的步骤是需要有效的营养培养基来积累李斯特菌病微生物。研究的目的。研制一种有利于李斯特菌团积累的有效营养培养基。材料和方法。以李斯特菌培养的实验培养基为研究对象。作为对照,我们用营养性琼脂(鱼粉水解液,fmh琼脂)和含1%葡萄糖的肉蛋白胨琼脂(MPA含1%葡萄糖)培养微生物。采用复合微生物学方法,对培养单核增生李斯特菌766过程中营养培养基的比活性进行了评价。结果。选择了培养李斯特菌的最佳培养基基质:河喜鹊胰腺水解液(Rutilus Rutilus lacustris)和肉制品废水水解液。开发了营养液的定性和定量组成,研究了营养液的物理、化学和生物特性。结果发现,在37°C条件下培养24小时后,该营养培养基提供了典型李斯特菌菌落的生长。发芽率为85%,比添加1%葡萄糖和GRM琼脂的MPA培养基的发芽率平均高21% (p < 0.05)。结论。培养李斯特菌的实验培养基使单核增生李斯特菌766菌落的生长保持了特有的培养、形态和生化特性,发芽率和生长速度均超过对照培养基。所开发的营养培养基为李斯特菌提供了有效的生长,可以作为微生物团块积累的培养基。
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Designing a Nutrient Medium for the Accumulation of Microbial Mass of Listeria
Background. To obtain reliable results of laboratory studies on the identification of Listeria, the presence of certified diagnostic agglutinating Listeria sera is required. An important step in the manufacturing process of such medical devices for in vitro diagnostics requires effective nutrient media for the accumulation of listeriosis microbe. Aim of the research. To develop an effective nutrient medium for the accumulation of bacterial mass of Listeria. Materials and methods. The object of the study was an experimental culture medium for Listeria cultivation. As a control, we used nutrient agar for the cultivation of microorganisms (fish meal hydrolysate, FMH-agar) and meat-peptone agar with 1 % glucose (MPA with 1 % glucose). The specific activity of nutrient media during cultivation of the test strain Listeria monocytogenes 766 was evaluated using a complex of microbiological methods. Results. The optimal base of the nutrient medium for Listeria cultivation has been selected: pancreatic hydrolysate of river magpie fish (Rutilus rutilus lacustris) and hydrolysate of meat water production waste. The qualitative and quantitative composition of the nutrient medium has been developed, its physical, chemical and biological properties have been studied. It was found that after 24 hours of incubation at 37 °C, the nutrient medium provided the growth of typical Listeria colonies. The germination rate was 85 %, which is higher compared to the growth of the culture on MPA with 1 % glucose and GRM agar by an average of 21 % (p < 0,05). Conclusion. The experimental culture medium for Listeria cultivation provided growth of colonies of the test strain L. monocytogenes 766 with the preservation of characteristic cultural, morphological and biochemical properties, and, in terms of germination and growth rate, exceeded the control media. The developed nutrient medium provides effective growth of Listeria and can be used as a medium for the accumulation of microbial mass.
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