用MALDI-TOF技术研究头孢西丁诱导产esbl大肠杆菌耐药蛋白的变化

Kamonlapob Boonrugsa, Kate Norkham, Siravit Chotimanon, Khetdan Panyadej, Rath Rerkasem, Pitchaya Singhavesjsakul, Ratchanee Somnabut, T. Sastraruji, S. Sookkhee
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摘要

摘要本研究旨在通过MALDI-TOF技术,解决2019-2020年清迈医院社区获得性尿路感染大肠埃希菌ESBL产AmpC酶的诊断问题,寻找头孢他啶单独暴露与ESBL抑制剂克拉维酸、AmpC诱导剂头孢西丁联合暴露的显著差异。经e条检测,254株大肠杆菌中有42.12% (n = 107)为高esbl产菌。6个峰的频率分别为2689(88.19%)、3126(90.55%)、6314(91.73%)、6411(88.98%)、7157(90.55%)、10301 (85.09%)Da,怀疑为大肠杆菌特异性肽谱。在高ESBL产生组中,三个具有统计学意义的肽谱只在4613 (13.33%,P = 0.008)、5613 (11.67%,P = 0.018)和9713 (55.00%,P < 0.001) Da被鉴定出来。3个以AmpC β-内酰胺酶方式作用的肽谱在该组分别为4184 (16.67%,P = 0.048)、9551 (10.00%,P = 0.021)和10477 Da (38.33%, P = 0.006),差异均有统计学意义。而非产生esbl组的AmpC肽谱分别为5380 (80.00%,P = 0.005)和6254 Da (66.67%, P = 0.016),具有统计学意义。结果表明,在头孢西丁诱导的一些高esbl和不产esbl的分离株中可以检测到AmpC酶相关光谱。关键词:AmpC, MALDI-TOF,头孢西丁,产esbl大肠杆菌,耐药蛋白
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Alteration of Drug-Resistant Proteins in ESBL-Producing Escherichia coli After Induction with Cefoxitin Using MALDI-TOF Technique
Abstract This study aimed to solve the diagnostic problem of AmpC enzyme production from ESBL production of community-acquired urinary tract-infected Escherichia coli from Maharaj Nakorn Chiang Mai Hospital in 2019-2020 by using the MALDI-TOF technique to search for the significant difference between the ceftazidime exposure alone and the concomitance of ESBL inhibitor, clavulanic acid, and AmpC inducer, cefoxitin. Among 254 E. coli isolates, 42.12% (n = 107) were categorized as high-ESBL producers after determined by E-strip test. The frequencies of six peaks, 2689 (88.19%), 3126 (90.55%), 6314 (91.73%), 6411 (88.98%), 7157 (90.55%), 10301 (85.09%) Da were suspected to be the E. coli specific peptide spectra. In the high-ESBL-producing group, three statistically significant peptide spectra which played an ESBL manner were only identified at 4613 (13.33%, P = 0.008), 5613 (11.67%, P = 0.018), and 9713 (55.00%, P < 0.001) Da. Three peptide spectra that acted in AmpC β-lactamase manner were statistically significant at 4184 (16.67%, P = 0.048), 9551 (10.00%, P = 0.021), and 10477 Da (38.33%, P = 0.006) in this group. Whereas the statistically significant peptide spectra which played as AmpC were identified at 5380 (80.00%, P = 0.005) and 6254 Da (66.67%, P = 0.016) in the non ESBL-producing group. Our results indicated that AmpC enzyme-related spectra could be detected in some high-ESBL and non ESBL-producing isolates after being induced by cefoxitin. Keywords: AmpC, MALDI-TOF, Cefoxitin, ESBL-producing E. coli, Drug resistance protein
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