Joshi Raghavendra, Janagama Harish, Dwivedi Hari P, Senthil Kumar T M A, Jaykus Lee-Ann, Schefers Jeremy, Sreevatsan Srinand
Veterinary Population Medicine Department, College of Veterinary Medicine, University of Minnesota, St. Paul, MN 55108, United States.
Mol Cell Probes. 2009 Feb;23(1):20-8. doi: 10.1016/j.mcp.2008.10.006. Epub 2008 Nov 18.
Sensitive and specific pre-analytical sample processing methods are needed to enhance our ability to detect and quantify food borne pathogens from complex food and environmental samples. In this study, DNA aptamers were selected and evaluated for the capture and detection of Salmonella enterica serovar. Typhimurium. A total of 66 candidate sequences were enriched against S. Typhimurium outer membrane proteins (OMPs) with counter-selection against Escherichia coli OMPs and lipopolysaccharides (LPS). Specificity of the selected aptamers was evaluated by gel-shift analysis against S. Typhimurium OMP. Five Salmonella-specific aptamer candidates were selected for further characterization. A dilution-to-extinction capture protocol using pure cultures of S. Typhimurium further narrowed the field to two candidates (aptamers 33 and 45) which showed low-end detection limits of 10-40CFU. DNase protection assays applied to these aptamers confirmed sequence-specific binding to S. Typhimurium OMP preparations, while South-Western blot analysis combined with mass spectrometry identified putative membrane proteins as targets for aptamer binding. Aptamer 33 was bound to magnetic beads and used for the capture of S. Typhimurium seeded into whole carcass chicken rinse samples, followed by detection using quantitative real-time RT-PCR. In a pull-down assay format, detection limits were 10(1)-10(2)CFU S. Typhimurium/9mL rinsate, while in a recirculation format, detection limits were 10(2)-10(3)CFU/25mL rinsate. Reproducible detection at <10(1)S. typhimurium CFU/g was also achieved in spike-and-recovery experiments using bovine feces. The pull-down analysis using aptamer 33 was validated on 3 naturally infected chicken litter samples confirming their applicability in the field. This study demonstrates the applicability of Salmonella specific aptamers for pre-analytical sample processing as applied to food and environmental sample matrices.
需要灵敏且特异的分析前样品处理方法,以提高我们从复杂食品和环境样品中检测和定量食源性病原体的能力。在本研究中,选择并评估了DNA适配体用于捕获和检测肠炎沙门氏菌鼠伤寒血清型。针对鼠伤寒沙门氏菌外膜蛋白(OMPs)富集了总共66个候选序列,并对大肠杆菌OMPs和脂多糖(LPS)进行反选。通过针对鼠伤寒沙门氏菌OMP的凝胶迁移分析评估所选适配体的特异性。选择了五个沙门氏菌特异性适配体候选物进行进一步表征。使用鼠伤寒沙门氏菌纯培养物的稀释至灭绝捕获方案进一步将范围缩小到两个候选物(适配体33和45),其显示出10 - 40CFU的低端检测限。应用于这些适配体的DNase保护试验证实了与鼠伤寒沙门氏菌OMP制剂的序列特异性结合,而蛋白质印迹分析与质谱联用鉴定了推定的膜蛋白作为适配体结合的靶标。适配体33与磁珠结合并用于捕获接种到全鸡胴体冲洗样品中的鼠伤寒沙门氏菌,随后使用定量实时RT-PCR进行检测。在下拉试验形式中,检测限为10(1)- 10(2)CFU鼠伤寒沙门氏菌/ 9mL冲洗液,而在再循环形式中,检测限为10(2)- 10(3)CFU / 25mL冲洗液。在使用牛粪的加标回收实验中也实现了在<10(1)鼠伤寒沙门氏菌CFU / g时的可重复检测。使用适配体33的下拉分析在3个自然感染的鸡粪样品上得到验证,证实了它们在实际应用中的适用性。本研究证明了沙门氏菌特异性适配体在应用于食品和环境样品基质的分析前样品处理中的适用性。
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