MicrobMatcher: a microbial comparison software based on matrix-assisted laser desorption/ionization with time-of-flight mass spectrometry

Matrix-assisted Laser Desorption/Ionization with Time-of-flight Mass Spectrometry (MALDI-TOFMS) was investigated as a method for the rapid identifica-tion of species. Current demand in microbial identi-fication is how to compare unknown strains to the known one quickly, semi-automatically and accurately. In this paper, we present a software tool that allows flexibly microbial matching in a user-friendly way, by letting the users to customize comparison parameters including: in vitro transcription enzyme, mass tolerance,minimum fragment length, intensity threshold and corresponding weights. We provide three spectral scoring functions to compute the affin-ity between the species. Therefore, the precision of microbial comparison increases. To test and verify this tool, we employed experimental spectral data based on MALDI-TOFMS and the gene sequences of E.coli and Salmonella. This software is written in Java for cross-platform intention.

Detection of Sialylated N-Linked Glycans by Matrix-Assisted Laser Desorption/Ionization Time-of-Flight Mass Spectrometry

Native and methyl-esterified sialylated glycans were analyzed with 2,4,6-trihydroxyacetophenone（THAP）and 2,5-dihydroxybenzoic acid（DHB）as matrix by a matrix-assisted laser desorption/ionization time-of-flight mass spectrometer（MALDI-TOF MS）.High quality negative-ion spectra of commercial sialylated glycan were obtained with THAP as matrix.Detection limit of the glycan was less than 0.1 pmol.After methyl esterification of sialic acid（SA）residue,sialylated glycans were detected sensitively in the positive-ion mode using DHB as matrix.Neutral and sialylated glycans from the mixture of asialofetuin and fetuin were methylesterified and simultaneously recognized in one manipulation.Methyl esterification of SA residue offers a convenient and sensitive way to identify the structure of N-linked glycans for glycan profiling.

MALDI-TOF MS直接靶板微滴生长测定法在CRKP快速检测中的应用

目的探讨基于基质辅助激光解吸电离飞行时间质谱(MALDI-TOF MS)的直接靶板微滴生长测定(DOT-MGA)法快速筛查碳青霉烯类耐药肺炎克雷伯菌(CRKP)的准确性和临床应用价值。方法收集2020—2021年连云港市第一人民医院肺炎克雷伯菌临床分离株251株,其中美罗培南敏感123株,CRKP128株。采用DOT-MGA法对4和6μL 2种取样量的所有菌株进行美罗培南耐药性检测。采用微量肉汤稀释法测定菌株的美罗培南最小抑菌浓度(MIC)。以微量肉汤稀释法耐药性分析结果为标准,评价DOT-MGA法耐药性检测结果的准确性。结果以微量肉汤稀释法为标准,孵育生长4 h后,DOT-MGA法2种取样量的敏感性和阴性预测值均为100.0%,其中4μL取样量检测CRKP的特异性为92.5%,阳性预测值为92.8%;6μL取样量检测CRKP的特异性为89.8%,阳性预测值为90.1%。123株美罗培南敏感株的美罗培南MIC_(50)为0.125μg·mL^(-1),MIC_(90)为0.25μg·mL^(-1);128株美罗培南耐药株的MIC_(50)和MIC_(90)均为≥128μg·mL^(-1)。DOT-MGA法与微量肉汤稀释法的一致性分析结果显示,4μL加样量Kappa值为0.88,6μL加样量Kappa值为0.83。结论基于MALDITOF MS的DOT-MGA法筛查CRKP具有较高的准确性,且简便、快捷,可用于快速检测CRKP。

MALDI-TOF MS法快速鉴定散装即食食品中3种食源性致病菌

本研究旨在利用基质辅助激光解吸电离飞行时间质谱法(Matrix-Assisted Laser Desorption Ionization-Time of Flight Mass Spectrometry,MALDI-TOF MS)快速检测并鉴定散装即食食品中的沙门氏菌、金黄色葡萄球菌和蜡样芽孢杆菌3种食源性致病菌。通过对点样方式、前处理方式、不同培养基及培养时间等各项实验条件的优化筛选确定最佳方法,并考察其检测限和稳定性,同时用所建立的方法与多重PCR法、VITEK 2等生化鉴定法进行结果比对,比较三者鉴定结果的一致性,最后进行批量食品样本检测来探寻MALDI-TOF MS鉴定法在散装即食食品中的适用性。结果表明,三种目标菌同一批次及不同传代次数的鉴定得分均大于95%,变异系数均小于2%,所建立的方法重复性和稳定性良好,且检测限为10^(5)CFU/mL,MALDI-TOF MS菌株鉴定结果与多重PCR法、生化鉴定法结果高度一致,且比二者检测用时更短,更加特异高效;在点样方式上,相较于夹心法与混合干滴法,三种覆盖法点样平均鉴定得分更高,均为99.9%,其中1μL+1μL覆盖法点样可获得的平均峰数目更多,特征峰更复杂且强度更高;而在前处理方式上,甲酸乙腈法与其他两种菌体处理方法相比可获得更多的出峰量和更高的峰强度,平均鉴定得分均在98%以上,且与数据库中图谱匹配度更高。综上所述,MALDI-TOF MS法在致病菌鉴定方面不仅灵敏特异、准确快速,且操作简便、结果直观,作为国标法的有力补充,为食源性致病菌的分析鉴定与分型溯源提供了新思路。

MALDI-TOF MS技术在临床微生物检验中的应用

随着科学技术的发展,新技术在医学检验中的应用越来越广泛。相较于传统微生物鉴定繁琐、耗时的工作流程,基质辅助激光解吸电离飞行时间质谱(MALDI-TOF MS,简称MS)技术因其快速、灵敏、简便、省时和特异性高等特点,在菌种鉴定、耐药监测、突变菌株鉴别等方面发挥巨大的作用,逐渐成为临床微生物实验室不可或缺的微生物鉴定工具。虽然MS技术鉴定菌种高度依赖数据库,也在一定程度上受限于临床样本质量,但其在临床微生物检验中仍有较大的空间待开发。文章对MS技术在临床微生物检验中的应用进行综述。

Identification of serum biomarkers for diagnosing stage Ⅰ lung adenocarcinoma by MALDI-TOF mass spectrometry

Objective To identify specific biomarkers that could improve early diagnosis of lung adenocarcinoma using matrix-assisted laser desorption/ionization (MALDI) technology. Methods Serum samples were isolated from 17 patients with stage Ⅰ lung adenocarcinoma and 17 age-and sex-matched healthy controls,and the serum proteomic profiles were obtained by matrix-assisted laser desorption ionization time of flight (MALDI-TOF) mass spectrometry. Results Compared with healthy control group,two highly expressed potential biomarkers were identified with the relative molecular weights of 6 631.64 Da and 4 964.21 Da. The two best novel protein peaks were automatically chosen for the system training and the development of the constructed model. The constructed model was then used to test an independent set of masked serum samples from 15 lung adenocarcinoma patients and 22 healthy individuals. The analysis yielded a sensitivity of 93.3%,and a specificity of 95.5%. Conclusion These results suggest that MALDI-TOF-MS ProteinChip technology is a quick,convenient,and high-output analyzing method that is capable of selecting several relatively potential biomarkers from the serum of lung adenocarcinoma patients and may have a clinical value in the future,and will provide clues to identifying new serologic biomarkers of lung adenocarcinoma.

MALDI-TOF-MS技术在肉芽肿性乳腺炎脓液棒状杆菌检测中的应用研究

目的:研究拟通过基质辅助激光解吸电离飞行时间质谱(MALDI-TOF-MS)技术在脓液克氏棒状杆菌(CK)鉴定过程中的应用探索,为临床微生物实验室对CK的准确鉴定提供帮助。方法:无菌条件下分别采集2019年1月-2021年7月镇江市妇幼保健院乳腺科门诊及病房30例经病理确诊为肉芽肿性乳腺炎(GM)患者手术中获取的新鲜脓肿穿刺液标本,用于细菌、真菌、结核菌涂片检查及需氧菌、厌氧菌培养。结果:采用梅里埃VITEK2compact全自动细菌鉴定仪进行生化鉴定,结果表明,23株菌鉴定为CK,其余7株菌均鉴定失败或错误。布鲁克MALDIBiotyper质谱仪鉴定结果27株为CK,仅3株菌鉴定失败,该结果与16SrRNA测序结果一致性较高,但是27份标本中鉴定为CK的质量分数相对较低。结论:MALDI-TOF-MS技术在棒状杆菌属细菌鉴定方面的应用可以为临床诊治GM方面提供病原学理论依据。

MALDI-TOF MS在血流感染快速鉴定病原菌中的应用

目的探讨基质辅助激光解吸电离飞行时间质谱(matrix-assisted laser desorption/ionization time of flight mass spectrometry,MALDI-TOF MS)结合短时培养在快速鉴定血流感染病原菌中的应用。方法对南京医科大学附属淮安第一医院微生物室2020年11月至2021年12月血培养报告阳性的标本进行革兰染色分类,并采用4h和6h短时培养法及MALDI-TOF MS技术快速鉴定感染病原菌并实时报送病区单元。结果4h短时培养革兰阴性菌共351株,339株(96.6%)细菌鉴定到种属,与24h鉴定结果相同,11株无鉴定结果,1株鉴定错误;6h短时培养革兰阳性菌共216株,212株(98.1%)鉴定到种属,与24h鉴定结果相同,3株无鉴定结果,1株鉴定错误。跟踪321株革兰阴性菌的临床反馈,287例(89.4%)给予临床关注,89例(27.7%)进行药物调整,238例(74.1%)临床疗效良好;跟踪183株革兰阳性菌的临床反馈,其中150例(82.0%)给予临床关注,49例(26.8%)进行药物调整,131例(71.6%)临床疗效良好。结论MALDI-TOF MS技术结合短时培养方法可有效提高血流感染病原菌鉴定准确率,改善血流感染患者抗菌药物治疗时机。

基于MALDI-TOF MS的血清多肽组学在胰腺良恶性疾病鉴别诊断中的应用

目的探讨基于基质辅助激光解吸电离飞行时间质谱(MALDI-TOF MS)的血清多肽组学在胰腺良恶性疾病鉴别诊断中的价值。方法选取胰腺导管腺癌(PDAC)患者176例、慢性胰腺炎(CP)患者148例,按7∶3的比例随机分成训练集(PDAC 122例、CP 103例)和验证集(PDAC 54例、CP 45例)。采用弱阳性离子交换法结合磁珠吸附提取血清多肽,采用MALDI-TOF MS检测多肽谱。在训练集中采用二分类Logistic回归分析建立基于差异表达多肽的PDAC和CP的鉴别诊断模型,并在验证集中进行验证。采用纳米液相色谱-电喷雾串联质谱(nano-LC/ESI-MS/MS)测定差异表达多肽的氨基酸序列,并鉴定其所属的蛋白质。采用受试者工作特征(ROC)曲线评价鉴别诊断模型鉴别PDAC和CP的效能,并与血清糖类抗原19-9(CA19-9)的鉴别诊断效能进行比较。结果共发现20个PDAC患者与CP患者之间有显著差异的多肽,依此建立的鉴别诊断模型鉴别PDAC和CP的曲线下面积(AUC)为0.988,最佳临界值为0.469,敏感性为94.26%,特异性为97.09%。在验证集中,该模型的敏感性为94.44%,特异性为97.78%;鉴别诊断模型效能优于血清CA19-9(敏感性为67.90%,特异性为91.30%)。鉴别诊断模型与CA19-9联合,鉴别PDAC和CP的AUC为0.996,敏感性为97.60%,特异性为100.00%。采用nano-LC/ESI-MS/MS成功鉴定出3种多肽所属蛋白质,m/z 1758为斑联蛋白片段,m/z 4053和m/z 5351均为纤维蛋白原片段。结论基于血清多肽组学建立的PDAC和CP鉴别诊断模型能较准确地区分胰腺良恶性疾病,为建立非侵入性肿瘤诊断方法提供了新思路。

Mass spectrometry-based serum peptide profiling in hepatocellular carcinoma with bone metastasis

AIM:To investigate the potential of serum peptides as a diagnostic tool for hepatocellular carcinoma(HCC)with bone metastasis.METHODS:Matrix-assisted laser desorption ionization-time of flight mass spectrometry(MALDI-TOF-MS)was used to characterize the serum peptide profile of HCC patients with bone metastasis.Serum samples from 138 HCC patients(66 cases with and 72 cases without bone metastasis)were randomly assigned into a training set(n=76)and a test set(n=62).Differential serum peptides were examined using ClinProt magnetic bead-based purification followed by MALDITOF-MS.The sequences of differentially expressed serum peptides were identified using liquid chromatography-mass spectrometry.A diagnostic model was established using a learning algorithm of radial basis function neural network verified by a single blind trial.Receiver operating characteristic(ROC)analysis was performed to evaluate the diagnostic power of the established model.RESULTS:Ten peptide peaks were significantly different between HCC patients with or without bone metastasis(P<0.001).Sequences of seven peptides with mass to charge ratios(m/z)of 1780.7,1866.5,2131.6,2880.4,1532.4,2489.8,and 2234.3 were successfully identified.These seven peptides were derived from alpha-fetoprotein,prothrombin,serglycin,isoform2 of inter-alpha-trypsin inhibitor heavy chain H4,isoform 1 of autophagy-related protein 16-2,and transthyretin and fibrinogen beta chains,respectively.The recognition rate and predictive power of a diagnostic model established on the basis of six significant peptides(m/z for these six peptides were 1535.4,1780.7,1866.5,2131.6,2880.4,and 2901.9)were 89.47%and82.89%,respectively.The sensitivity and specificity of this model based upon a single blind trial were 85.29%and 85.71%,respectively.ROC analysis found that the AUC(area under the ROC curve)value was 0.911.CONCLUSION:Our study suggested that serum peptides may serve as a diagnosis tool for HCC bone metastasis.

Establishment and Preliminary Application of Two dimensional Electrophoresis and Mass Spectrometry in Ovary Study

Objective To apply two-dimensional electrophoresis and mass spectrometry in the ovary proteome researchMethods Protein extractions from mouse ovaries were run in IPGphor isoelectric focus system with 11 cm and 24 cm IPG strips respectively (pH 3～10, 0.3 mm thick), then the protein spots were identified by mass spectrometry.Results The ovary protein exactions separated by two-dimensional electrophoresis have got high resolution, and identifing protein by mass spectrometry was highly efficient and facilitly. These two techniques should facilitate further investigation of female reproduction proteome research.Conclusion These two rapid high resolutions and efficient techniques have a variety of applications foreground in female reproduction proteome pattern research.

MALDI-TOF质谱技术对猪肠道菌群中携带mcr-1细菌的鉴定与聚类分型

为了解多粘菌素耐药基因mcr-1在猪肠道微生物群落中的分布特征,本研究采集分离同一猪肠道样品中的多粘菌素耐药菌,利用PCR进行mcr-1基因检测,采用基质辅助激光解析电离飞行时间质谱(MALDI-TOF MS)技术对mcr-1阳性菌株进行种属鉴定与亲缘关系分析。结果显示,在收集获得的325株多粘菌素耐药菌中,136株(41.8%)含有mcr-1基因,包括大肠杆菌70株,肺炎克雷伯菌19株,放线杆菌47株。细菌蛋白指纹图谱进行聚类分析显示,70株mcr-1阳性大肠杆菌被划分为13个亚型,19株肺炎克雷伯菌被分为3个亚型,其中有17株菌属于同一亚型(占89.5%),47株放线杆菌均为同一克隆。上述结果表明mcr-1在肠道菌群中存在克隆传播现象,细菌指纹图谱的多样性也提示可能存在质粒或者其他转移元件介导的mcr-1水平传播。MALDI-TOF-MS作为一种新的技术,不仅能够实现细菌的快速鉴定,而且可基于细菌蛋白指纹图谱对菌株进行初步的亲缘关系分析。

MALDI-TOF-MS技术应用于消化道肿瘤蛋白组学的研究进展

基质辅助激光解吸电离飞行时间质谱(matrix-assisted laser desorption ionization time-of-flight mass spectrometry, MALDI-TOF-MS)技术作为一种生物质谱技术,可广泛应用于基因突变检测、基因多态性研究、微生物鉴定、肿瘤生物学标志物检测等方面,其对于早期疾病的发现、治疗以及评估预后有着重要指导意义,已成为精准医学领域不可缺少的分子诊断技术。本文对MALDI-TOF-MS技术在消化道肿瘤蛋白质组学的应用方面进行综述。

氮掺杂芦丁基碳点作为MALDI-TOF-MS基质对氨基酸的检测

以芦丁为碳源、乙二胺为氮源,采用水热法制备氮掺杂芦丁基碳点(N-CD)。通过优化温度、时间、碳源质量等反应条件得到N-CD荧光最大值。将N-CD作为基质辅助激光解吸电离飞行时间质谱(MALDI-TOF-MS)基质对氨基酸进行检测。结果显示:氮原子在N-CD中主要以吡啶氮形式存在,氮原子的孤电子对与碳点的sP2芳香体系以垂直形式构成的共轭结构,增大了共结晶电子解吸/电离效率。使用N-CD对谷氨酸、组氨酸、苯丙氨酸和天冬氨酸进行检测。检测结果表明氨基酸离子信号强度最高可达30382。N-CD溶液作为基质最佳质量浓度为0.5 mg/mL,最大耐盐度为1 mol/L,初步实现对人体血清中氨基酸进行高通量检测。N-CD作为MALDI-TOF-MS新型基质材料在分析化学检测、环境检测以及生物小分子检测中具有良好的应用潜力,也为多元素掺杂生物质碳点材料作为MALDI-TOF-MS基质提供了参考。

MALDI-TOF MS技术检测胃癌患者外周血中miR-34b/c甲基化及临床意义

目的探讨胃癌患者外周血中miR-34b/c启动子区甲基化状态及临床意义。方法采用基质辅助激光解吸电离飞行时间质谱(matrix-assisted laser desorption/ionisation,time-of-flight mass spectrometry,MALDI-TOF MS)技术检测31例胃癌患者和24例正常人群外周血中miR-34b/c启动子区甲基化状态,筛选与胃癌发生相关的差异性甲基化CpG位点,并分析其与胃癌临床病理特征的相关性。14 C尿素呼气试验(UBT)检测胃癌患者HP感染状态,分析其与miR-34b/c甲基化的相关性。免疫组化EnVision两步法检测胃癌组织中MMR蛋白表达,分析其与miR-34b/c甲基化的相关性。结果胃癌中miR-34b/c整体甲基化水平高于正常对照组,其中3个CpG单位CpG_3.4、CpG_20、CpG_25在胃癌中的甲基化水平(13.61%、11.32%、15.32%)明显高于正常对照组(2.36%、0.41%、7.60%),差异有显著性(P<0.01)。进一步分析CpG位点与临床病理特征的关系,发现miR-34b/c CpG_3.4高甲基化与胃癌淋巴结转移相关(P<0.05),而miR-34b/c CpG_3.4、CpG_20、CpG_25高甲基化与患者年龄、性别、发病部位、分化程度、TNM分期无相关性(P>0.05)。31例胃癌患者HP感染阳性检出率为51.61%(16/31)。HP感染与miR-34b/c高甲基化无相关性(P>0.05)。31例胃癌患者中,错配修复基因缺失(deficient mismatch repair,dMMR)2例(6.45%),错配修复基因完整(proficient mismatch repair,pMMR)29例(93.55%)。MMR蛋白表达与miR-34b/c高甲基化无相关性(P>0.05)。结论miR-34b/c启动子区高甲基化改变可能在胃癌的发生、发展中发挥重要作用,并可作为胃癌诊断和预后预测的潜在生物学标志物。

MALDI-TOF MS技术在真菌鉴定和药敏试验中的影响因素研究

基质辅助激光解吸电离飞行时间质谱(MALDI-TOF MS)是一种具有经济、快速、准确、高通量等特点的新技术,广泛应用于临床微生物的常规鉴定。近年来,随着MALDI-TOF MS技术的不断发展,其在临床感染性真菌的快速鉴定、药敏试验、分型等实验室诊断中在一定程度上弥补了传统形态学鉴定的不足,展现出巨大的应用潜力。由于真菌种类繁多、结构复杂、耐药谱多样及表型可变,在MALDI-TOF MS技术分析真菌的过程中,影响因素相对来说比较复杂,该文就不同培养条件、蛋白质提取方法和蛋白图谱数据库等条件对MALDI-TOF MS技术鉴定真菌的影响作一综述。

MALDI-TOF MS在不同禽肉动物源性成分检测中的研究

[目的]建立基质辅助激光解吸电离飞行时间质谱(matrix-assisted laser desorption ionization-time of flight mass spectrometry, MALDI-TOF MS)技术检测不同禽肉动物源性成分的方法,构建不同禽肉蛋白质分子指纹图谱标准数据库,对不同禽肉进行鉴别。[方法]样品用磷酸盐缓冲液提取,净化后用MALDI-TOF MS法测定。采用ChemPattern软件对不同禽肉蛋白图谱进行化学计量学分析,建立识别模型。[结果]鸡、鸭、鹅3种不同禽肉之间具有明显差异。首次建立不同禽肉蛋白质分子指纹图谱标准数据库,可一次性对每个样品中鸡、鸭、鹅等肉源性成分进行同时分析。[结论]建立的基于蛋白质组学的鸡、鸭、鹅源性成分鉴定系统具有简便、稳定、准确、重现性好的优点,适用于不同禽肉中鸡鸭鹅动物源性成分的鉴别。

MALDI-TOF MS快速检测血流感染大肠杆菌对第3代头孢菌素的药敏研究

目的评价基质辅助激光解析电离飞行时间质谱(matrix-assisted laser desorption ionization-time of flight,MALDI-TOF MS)直接靶板微滴生长法(direct-on-target microdroplet growth assay,DOT-MGA)快速检测血流感染大肠杆菌对第3代头孢菌素药敏实验的价值。方法收集血流感染大肠杆菌50株作为实验菌株。采用菌液与不同浓度头孢噻肟在靶板上混合作为检测孔,不加抗菌药物的菌液作为生长对照孔,孵育4h后,根据DOT-MGA法鉴定靶板上的待测菌,所对应检测孔位代表头孢噻肟最低抑菌浓度,并以微量肉汤稀释法作为比较。结果微量肉汤稀释法和DOT-MGA法检测大肠杆菌对头孢噻肟最低抑菌浓度基本一致率为96%,分类一致率为94%,较大偏差为2%,次要偏差为4%,未发现重大偏差,均在临床可接受范围内。结论MALDI-TOF MS结合DOT-MGA法能够短时间内准确提供大肠杆菌对第3代头孢菌素的药敏信息,为临床早期精准管理血流感染患者提供依据。

磁性氮化碳复合材料的制备及其对磷酸化肽的富集

蛋白质的磷酸化在细胞信号传导和疾病发生发展中起着重要作用,但磷酸化的动态变化和低丰度的特点使得对其直接分析有着较大的困难。为了解决磷酸化肽难离子化、检测丰度低的瓶颈问题,本研究制备了一种磁性氮化碳复合材料,结合基质辅助激光解吸电离飞行时间质谱(MALDI-TOF-MS),建立了一种对复杂样品中低丰度磷酸化肽富集与分析的方法。采用电子显微镜、红外光谱分析及X射线衍射分析等手段对合成的磁性氮化碳材料进行表征。以酪蛋白酶解产物为实验模型,发现磁性氮化碳材料能够实现对磷酸化肽的高选择性富集和高灵敏度检测,检出限为0.1 fmol。选择脱脂牛奶、人唾液和人血清为实际分析样品,发现磁性氮化碳材料对微量蛋白生物样品中磷酸化肽的分析具有较高的应用潜力。