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.

Rapid Profiling of Alkaloids in Several Medicinal Herbs by Matrix-assisted Laser Desorption/Ionization Mass Spectrometry

A simple method was developed for rapid and direct profiling of alkaloids in medical herbs via matrix-assisted laser desorption/ionization time-of-flight mass spectrometry（MALDI-TOF MS）. The dry herbs were first ground to powder and passed through a stainless steel sieve, mixed with the matrix solution to form a homogeneous suspension, which was then directly applied to MALDI analysis. Several matrices were investigated and 2,5- dihydroxybenzoic acid（DHB） was chosen as the optimized one, and the particle with small size was found to favor the analysis. Using this method, the profiles of alkaloids in several medical herbs were readily obtained, and the toxicities of crude and processed Radix Aconiti Lateralis Preparata were compared via the relative intensities of the peaks of the corresponding toxic components shown in their MALDI spectra. This method therefore provides a rapid and reliable protocol for obtaining profiles of alkaloids in medical herbs by using MALDI-TOF MS.

A novel sample preparation method of matrix-assisted laser desorption/ionization time of flight mass spectrometry for polystyrene

A novel sample preparation method of matrix-assisted laser desorption/ionization mass spectrometry for polystyrene was reported. Compared to the conventional dried-droplet method, the efficiency of ionization and signal intensity of mass spectra were improved. The mechanism was also analyzed.

Detection of lung adenocarcinoma using magnetic beads based matrix-assisted laser desorption/ionization time-of-flight mass spectrometry serum protein profiling

Background Recently, due to the rapid development of proteomic techniques, great advance has been made in many scientific fields. We aimed to use magnetic beads （liquid chip） based matrix-assisted laser desorption/ionization time-of-flight mass spectrometry （MALDI-TOF-MS） technology to screen distinctive biomarkers for lung adenocarcinoma （adCA）, and to establish the diagnostic protein profiles. Methods Using weak cation exchange magnetic beads （MB-WCX） to isolate and purify low molecular weight proteins from sera of 35 lung adCA, 46 benign lung diseases （BLDs） and 44 healthy individuals. The resulting spectra gained by anchor chip-MALDI-TOF-MS were analyzed by ClinProTools and a pattern recognition genetic algorithm （GA）. Results In the working mass range of 800-10 000 Da, 99 distinctive peaks were resolved in lung adCA versus BLDs, while 101 peaks were resolved in lung adCA versus healthy persons. The profile gained by GA that could distinguish adCA from BLDs was comprised of 4053.88, 4209.57 and 3883.33 Da with sensitivity of 80%, specificity of 93%, while that could separate adCA from healthy control was comprised of 2951.83 Da and 4209.73 Da with sensitivity of 94%, specificity of 95%. The sensitivity provided by carcinoembryonic antigen （CEA） in this experiment was significantly lower than our discriminatory profiles （P 〈0.005）. We further identified a eukaryotic peptide chain release factor GTP-binding subunit （eRF3b） （4209 Da） and a complement C3f （1865 Da） that may serve as candidate biomarkers for lung adCA. Conclusion Magnetic beads based MALDI-TOF-MS technology can rapidly and effectively screen distinctive proteins/polypeptides from sera of lung adCA patients and controls, which has potential value for establishing a new diagnostic method for lung adCA.

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.

Matrix-assisted laser desorption/ionization time of flight mass spectrometry in the genetic basis of systemic lupus erythematosus and the complicating kidney injury

Background It is necessary to develop some innovative methods to reveal and discover the novel （SLE）-related protein molecules. In the present study, matrix-assisted laser desorption/ionization time of flight mass spectrometry （MALDI- TOF MS） was employed to detect the differential expression of serum polypeptides in the patients with systemic lupus erythematosus （SLE） presenting with a family history or complicating with kidney injury so as to identify the proteins associated with the genetic factors and kidney injury in SLE. Methods The subjects recruited were divided into four groups, that is, a group of SLE patients with both family history and kidney injury, a group of SLE patients with only kidney injury but no family history, a group of SLE patients with neither family history nor kidney injury, and a control group consisting of healthy volunteers. By adopting MALDI-TOF MS analysis, the serum samples obtained from the three groups of SLE patients were examined and compared with those from the control group; the categorized peptide fingerprint profile was established via the biological data collected from the samples. Results The expression of protein with a mlz of 4207 Da increased significantly in SLE patients; the protein with a ml z of 2658 Da was expressed in all SLE patients; three proteins （with mlz of 1465, 5332, and 5900 Da respectively） were expressed in the SLE patients complicated with kidney injury and the protein with a mlz of 1943 Da was expressed in SLE patients with family history. Conclusion A number of differential proteins were successfully detected and identified through MALDI-TOF MS detection and these proteins may be associated with the genetic basis of SLE and the complicating kidney injury.

核酸MALDI-TOF MS检测在肺结核诊断中的价值

目的探讨基质辅助激光解吸电离飞行时间质谱(MALDI-TOF MS)在疑似肺结核(PTB)诊断中的应用价值及其阳性结果的影响因素,以期为临床治疗提供参考。方法选取甘肃省第二人民医院(西北民族大学附属医院)2022年8月—2023年3月收治的疑似PTB患者77例为研究对象。所有患者肺泡灌洗液(BALF)均接受MALDI-TOF MS检测和结核分枝杆菌(MTB)培养。根据MTB培养结果,对核酸MALDI-TOF MS检测进行诊断效能分析,并探讨核酸MALDI-TOF MS检测阳性的影响因素。结果核酸MALDI-TOF MS检测结果显示,MTB阳性共37例(48.1%,37/77),40例阴性(51.9%,40/77)。以培养结果为金标准,核酸MALDI-TOF MS的灵敏度、特异度、阳性预测值(PPV)、阴性预测值(NPV)和准确度分别为90.9%、84.1%、81.1%、92.5%和87.0%,采用Kappa检验法评价核酸MALDI-TOF MS检测和MTB培养法的一致性,结果显示Kappa值为0.739(P<0.05)。2组患者在是否有糖尿病、身体质量指数(BMI)及降钙素原(PCT)方面比较,差异均有统计学意义(P<0.05)。多因素Logistic回归分析结果显示:有糖尿病和PCT异常为核酸MALDITOF MS阳性的独立危险因素(P<0.05)。结论核酸MALDI-TOF MS检测对PTB的早期诊断具有重要价值,可为患者的规范用药提供更好的指导,即为患者的治疗制定更为精准、有效的治疗方案,从而提高治疗效果、改善患者生活质量。

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。

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。

分离胶促凝管联合MALDI-TOF MS直接检测血培养阳性细菌

目的建立用分离胶促凝管联合基质辅助激光解析电离飞行时间质谱（MALDI-TOF MS）直接检测血培养阳性待测菌的方法并评估其鉴定符合率。方法共收集阳性血培养491例,利用分离胶促凝管直接从血培养瓶中富集并提纯菌体,采用MALDI-TOF MS对待测菌进行菌种鉴定,同时对报阳性血培养瓶进行转种培养,纯菌落用Vitek 2 Compact全自动微生物分析系统（简称Vitek 2 Compact）进行鉴定。若两者鉴定结果不一致,则以基因测序结果予以确证。结果 491例阳性血培养瓶鉴定出的待测菌包括30个属和64个种。在462例单菌株感染血培养瓶中,菌株的种、属鉴定符合率分别为73.6%和3.7%。其中175例革兰阴性菌的种、属鉴定率分别为84.0%（147例）和2.9%（5例）;251例革兰阳性菌的种、属鉴定率分别为75.3%（189例）和4.4%（11例）;36例念珠菌的种、属鉴定率分别为19.4%（7例）和2.8%（1例）。在29例复数菌感染血瓶中,鉴定出其中一种细菌的种、属鉴定率分别为79.3%（23例）和10.3%（3例）。血流感染中常见病原菌的菌种鉴定符合率达83.3%～96.9%。结论本研究建立了分离胶促凝管联合MALDI-TOF MS直接检测血培养阳性待测菌的方法,与传统的培养鉴定方法相比,对血流感染中主要病原菌的鉴定符合率较高,且方法快速、简便,成本低廉,适合在临床微生物实验室中推广应用。

Microflex^(TM) MALDI-TOF MS和Vitek 2 Compact全自动微生物分析系统对肠杆菌科细菌鉴定能力的比较

目的比较MicroflexTM基质辅助激光解吸电离飞行时间质谱(MALDI-TOF MS)和Vitek 2 Compact全自动微生物分析系统(简称Vitek 2 Compact)对肠杆菌科细菌的鉴定能力。方法采用MicroflexTMMALDI-TOF MS和Vitek 2 Compact同时对545株肠杆菌科质控菌株和临床分离菌株进行鉴定,鉴定结果不一致者采用沙门菌血清凝集试验或细菌16S r DNA基因测序予以确证。结果 MicroflexTMMALDI-TOF MS对545株细菌的种和属的鉴定率分别为97.1%、2.9%。Vitek 2 Compact对545株细菌的种、群、属的鉴定率分别为83.3%、13.9%和2.2%,鉴定错误率为0.2%,未鉴定率为0.4%。结论 MicroflexTMMALDI-TOF MS对肠杆菌科细菌的鉴定符合率高于Vitek 2 Compact,且操作快速、简便,成本低,可用于临床肠杆菌科细菌的常规快速鉴定。

MALDI-TOF MS与16SrDNA方法对肠杆菌科微生物鉴定比较分析

为了研究基质辅助激光解吸电离飞行时间质谱(MALDI-TOF MS)法鉴定肠杆菌科微生物及其对微生物系统分类学相关分析的准确性,采用MALDI-TOF MS对金桔表面分离的10种肠杆菌科微生物进行蛋白质图谱收集,通过比对图谱特征峰实现微生物的鉴定与系统进化学分析;同时对10种微生物进行16SrDNA提取与测序,得到分子生物化学水平鉴定,并采用邻近连接法对16SrDNA序列做系统进化树分析。结果表明:MALDI-TOF MS与16SrDNA测序对10种肠杆菌科微生物鉴定结果中,克雷伯菌属2株菌鉴定种级有偏差,其他8种一致;MALDI-TOF MS与16SrDNA测得的数据都可计算微生物相关性,从而得到微生物系统发育树,两株系统发育树中同属级微生物归类的亲缘位置与方向一致,但不同属肠杆菌科微生物的亲缘距离与位置差异较大。MALDI-TOF MS法鉴定农产品表面微生物具有快速、准确的特点,但准确建立系统发育相关性还需要扩大数据库和优化算法。

MALDI-TOF MS结合短期培养法快速检测中段尿样本中的病原菌

目的探讨基质辅助激光解析电离飞行时间质谱(MALDI-TOF MS)结合短期培养法快速检测中段尿样本中病原菌的价值。方法收集1 873例患者的中段尿样本,每份样本一分为二,一份用于中段尿常规培养结合Vitek 2 Compact微生物鉴定仪检测;另一份样本离心集菌后,短期培养4或6 h,采集菌膜直接用MALDI-TOF MS进行鉴定,并以中段尿定量培养结合Vitek 2 Compact微生物鉴定仪的检测结果为金标准,评估MALDI-TOF MS结合短期培养法对尿路感染病原菌鉴定的敏感性及特异性。结果在1 873例临床样本中常规培养方法检出病原菌381例,阳性检出率为20.3%。其中单一细菌生长的样本346例(90.8%),2种细菌生长的样本27例(7.1%),3种及3种以上细菌生长的样本8例(2.1%)。在单一细菌生长的样本中,短期培养4 h后MALDI-TOF MS直接检测的检出率为80.1%(277/346),短期培养6 h后MALDI-TOF MS直接检测的检出率为97.1%(336/346)。除鲍曼不动杆菌、屎肠球菌和粪肠球菌鉴定符合率稍低(81.4%、76.9%和86.7%)外,MALDI-TOF MS结合6 h短期培养法的鉴定符合率均为100.0%。结论将中段尿样本离心集菌后短期培养4~6h,采集菌膜直接用MALDI-TOF MS进行检测,可大大缩短培养时间,为临床提供快速的病原菌报告。

MALDI-TOF MS和电子光谱技术研究海兔肝铁蛋白亚基电离和释放铁动力学特性

选用肽质量指纹谱(peptide mass fingerprint,PMF)技术鉴定质谱纯海兔肝铁蛋白(liver ferritin ofAplysia,ALF)。来源于基质辅助激光解吸电离飞行时间质谱(MALDI-TOF MS)仪中的激光和基质芥子酸协同解吸海兔肝铁蛋白(ALF)为带双电荷、单电荷[M+H]+和二聚体的亚基离子,并可供质谱分析。ALF亚基的质荷比m/z分别为9784.03[M+2H]2+、19678.42[M+H]+和39387.80[2M+H]+,其中亚基分子量[M+H]+略小于鲨鱼肝铁蛋白(liver ferritin of shark,SLF)。在弱碱介质(pH8.0)条件下,电子光谱技术研究指出,抗坏血酸以1/2级反应方式参与ALF释放铁全过程,同时又使ALF以一级反应动力学方式释放铁,呈现两种不同的速率。推测这一异常现象可能与ALF含低铁量、亚基调节能力和海兔的进化地位有关。

MALDI-TOF MS磷脂质组学快速分析三文鱼肌肉组织

建立了基质辅助激光解吸电离-飞行时间质谱(MALDI-TOF MS)快速分析三文鱼肌肉组织磷脂质组学的方法。以非自然磷脂酰胆碱DMPC(14∶0/14∶0)和磷脂酰乙醇胺DPPE(15∶0/15∶0)为标准品,分析其在正离子模式下的主要分子峰与干扰峰,并进行方法学验证。实验结果表明,各化合物平均加标回收率在74%~83%之间,相对标准偏差小于7%,日内和日间精密度的相对标准偏差均低于8.5%。将三文鱼磷脂提取物进样分析,共鉴定出28种磷脂分子,其中m/z806.40([PC38:6+H]^+和[PE38:4+K]^+)信号最强。三文鱼中多不饱和磷脂种类丰富,如m/z 824.38([PC38:8+Na]^+和[PE42:5+H]^+),m/z832.41([PC40:7+H]^+,[PC38:4+Na]^+和[PE40:5+H]^+),部分磷脂分子的脂肪酸链达到了满不饱和,如[PC42:11+H]^+,其sn-1和sn-2上两条脂肪酸链分别为二十碳五烯酸链(EPA-)和二十二碳六烯酸链(DHA-)。该方法稳定可靠,可用于鉴定三文鱼肌肉组织中的磷脂分子结构,并从脂质组学角度为三文鱼营养评价提供理论依据。

MALDI-TOF质谱技术鉴定龋病患者唾液中的变异链球菌

目的:利用基质辅助激光解吸电离时间飞行质谱(matrix-assisted laser desorption/ionization time-of-flight mass spectrometry,MALDI-TOF MS)鉴定龋病患者唾液中的变异链球菌,为探寻快速、准确鉴定变异链球菌的方法提供依据。方法:研究对象为北京大学口腔医院牙体牙髓科就诊的90名龋病患者,收集受试者的唾液样本,处理后进行MALDI-TOF MS检测,结果导入BioExplorer 1.0软件与标准库比对,分值≥25者鉴定为变异链球菌,<25者鉴定为非变异链球菌。最后将质谱和16S rDNA测序结果进行比对,计算灵敏度和一致率。结果:MALDI-TOF MS鉴定变异链球菌的灵敏度为96.0%,与16S rDNA测序结果的一致率为98.7%。结论:MALDI-TOF MS是一种高通量、快速且操作简便的方法,鉴定变异链球菌的灵敏度和一致率都很高,具有较高的临床应用价值。

MALDI-TOF MS分析研究合成高分子的综述

扼要介绍了基质辅助激光解吸电离/飞行时间质谱,在分析合成高分子中的发展历程、基本原理、主要优点及存在的困难;详细分析了基质、溶剂、盐（阳离子）和样品制样方法等关键因素对实验结果的影响及造成质量歧视的原因;阐明了这一分析技术在均聚物、混合物、共聚物等合成高分子研究中的应用及展望。

MALDI-TOF-MS在病原微生物鉴定中的研究进展

基质辅助激光解吸电离飞行时间质谱(MALDI-TOF-MS)是鉴定多种致病性细菌的快速、可靠的方法,具有较好的稳定性和可重复性,在快速和准确性方面的总体表现明显好于传统的细菌生化鉴定方法。适合于一些致病菌的快速、高通量的检测和鉴定。综述MALDI-TOF-MS技术在普通病原菌、多血清型病原菌、非发酵性细菌,以及植物病原菌等病原微生物鉴定方面的最新研究进展。