采用SELDI蛋白质芯片技术研究氧化亚铁硫杆菌对磷酸盐缺失的反应

氧化亚铁硫杆菌(At.f)是能够利用Fe2 和硫化矿来获取能量的一种化能自养菌.这种细菌在金属硫化矿的生物浸出中起着重要的作用.在硫化矿的生物浸出过程中,浸矿细菌通常会遇到多种胁迫条件,如温度的变化、营养成分的缺失和pH值的变化等,这些因素会影响到细菌的活性.因此对在胁迫条件下这类细菌的应急反应生理机制的研究具有重要的意义.SELDI蛋白质芯片技术是近年一种高通量的蛋白质组学研究技术.测定了以Fe2 为能源正常条件培养的At.f和磷酸盐缺失培养At.f的生长情况,绘制了相应的生长曲线;采用NP20蛋白质芯片,对At.f总蛋白的蛋白质芯片上样量进行了优化.在此基础上,采用IMAC-Cu、SAX2、WCX2三种特异性SELDI蛋白质芯片技术,获取了磷酸盐缺失培养At.f与正常条件培养的At.f的比较蛋白质图谱,采用软件对比较蛋白质图谱进行分析,发现了磷酸盐缺失培养At.f的13个明显差异表达的蛋白质分子,为进一步分离鉴定这些差异表达蛋白质奠定了基础.     

应用蛋白质芯片技术从血清中筛选肺癌标志蛋白

探讨用蛋白质芯片技术筛选肺癌病人血清中的特异性标志蛋白. 采用SELDI (surfaced enhanced laser desorption/ionization)蛋白芯片技术检测了30例肺癌(15例原发癌, 9例转移癌, 6例化疗后)病人血清和12例正常人血清中的蛋白质谱. 选用阴离子交换柱处理血清样品, 用5个不同pH的洗脱液和有机溶剂洗脱柱床, 通过改变洗脱液的pH值得到6个具有不同pI的蛋白质组分. 每个组分用IMAC-Cu和WCX2两种芯片检测. 采用美国Ciphergen 生物公司研制的蛋白质芯片阅读机读取数据, 获得的蛋白质谱采用Ciphergen 公司的Biomark Wizard软件分析. 结果显示, 肺癌病人与正常人的血清中有15个差异蛋白(标志分子)表达. 与正常人血清相比, 6个蛋白质在肺癌病人血清中高表达, 9个蛋白质在肺癌病人血清中低表达. 采用单一标志分子检测时, 敏感性为44.82%~93.1%, 特异性为85%~94.4%. 其中5个标志分子在两种芯片上被检测出来. 实验证明与肺癌相关的特异性标志分子可从病人血清中检测出来, 而且蛋白质芯片技术对于发现和筛选血清中的肺癌标志蛋白是一种有效、快速的工具.     

尿样在SELDI技术中的优化研究

目的：建立表面增强激光解吸离子化飞行时间质谱（SELDI．TOF／MS）技术检测尿液样本的方法。方法：采用SELDI技术及弱阳离子交换表面蛋白芯片（CM10）对糖尿病病例组和正常对照组的尿液样本进行分析,从尿液标本的采集、样品保存、上样浓度的控制、实验仪器的内外校准、实验结果重复性验证与分析等方面进行实验条件的优化。结果：反复冻融3次以上的样品经SELDI检测的出峰数量和峰强度情况较差;以1：1或1：2的浓度作倍比稀释后的样本经芯片检测得到的蛋白峰强度和蛋白数量最优;对两组样本重复检测3次,蛋白丰度的平均变异系数（CV值）分别为0．121和0．095;两组样本共检测到202个蛋白峰,其中差异表达蛋白29个,在肝纤维化组中表达上调13个,表达下调16个。结论：初步建立了SELDI技术检测尿液样本的方法,提高了SELDI技术检测尿液样本的质量。     

电针对大鼠胃黏膜损伤修复的血清蛋白质差异表达研究

目的：观察电针胃经穴对大鼠胃黏膜损伤修复的血清蛋白质差异表达,为进一步阐明针刺效应的体液机理提供理论依据。方法：用表面增强激光解吸离子化飞行时间质谱（SELDI—TOF—MS）技术和WCX2（弱阳离子交换芯片）对正常大鼠血清和电针大鼠血清进行蛋白质指纹图谱检测分析,通过Biomarker Wizard和Biomarker Patterns System软件判别分析处理数据并结合生物信息学方法筛选差异表达蛋白质。结果：与正常大鼠血清比较,电针大鼠血清蛋白质在质荷比为2000-50000有25个蛋白质峰差异有显著意义,其中有19个标志蛋白在电针胃经大鼠血清中呈现高表达,6个标志蛋白在电针胃经大鼠血清中呈现低表达。结论：电针可促进胃黏膜损伤大鼠血清蛋白质差异表达,这种差异蛋白质可能与电针促进胃黏膜损伤修复效应密切相关。     

尿样在SELDI技术中的优化研究

目的:建立表面增强激光解吸离子化飞行时间质谱(SELDI-TOF/MS)技术检测尿液样本的方法。方法:采用SELDI技术及弱阳离子交换表面蛋白芯片(CM10)对糖尿病病例组和正常对照组的尿液样本进行分析,从尿液标本的采集、样品保存、上样浓度的控制、实验仪器的内外校准、实验结果重复性验证与分析等方面进行实验条件的优化。结果:反复冻融3次以上的样品经SELDI检测的出峰数量和峰强度情况较差;以1:1或1:2的浓度作倍比稀释后的样本经芯片检测得到的蛋白峰强度和蛋白数量最优;对两组样本重复检测3次,蛋白丰度的平均变异系数(CV值)分别为0.121和0.095;两组样本共检测到202个蛋白峰,其中差异表达蛋白29个,在肝纤维化组中表达上调13个,表达下调16个。结论:初步建立了SELDI技术检测尿液样本的方法,提高了SELDI技术检测尿液样本的质量。     

大肠埃希菌蛋白指纹图谱的建立

目的建立大肠埃希菌（Escherichia coli,E．coli）蛋白指纹图谱,为Ecoli感染快速诊断奠定基础。方法收集临床分离E.coli88株,提取细菌DNA,PCR检测Ecoli 16S rRNA。蛋白提取液提取细菌蛋白,干化学法测蛋白浓度,应用表面增强激光解析电离飞行时间质谱技术（SELDI-TOF-MS）检测Ecoli蛋白,采用Ciphergen Pro-teinchip软件自动采集数据。重复测定20次Ecoli混合标本,评价SELDI检测Ecoli蛋白分子量的重复性。结果E．coil标准菌株ATCC 25922和临床分离株均可检出16S rRNA。AU芯片能捕获近30个E．coli蛋白峰,其中19个蛋白峰构成E．coli特征性蛋白指纹图谱,各蛋白峰在临床分离E．coli间分子量变异系数≤0．2％。SELDI重复检测20次E．coli混合标本显示同一蛋白峰的分子量变异系数≤0．05％。结论E．coli在分子量3～20kD范围内具有特征性蛋白指纹图谱,为快速诊断E.coli感染提供了新思路。     

分枝杆菌特征性蛋白的筛选

目的研究分枝杆菌蛋白表达,筛选分枝杆菌特征性蛋白,为分枝杆菌的快速鉴定奠定基础。方法选取分枝杆菌标准菌株,提取细菌蛋白,干化学法测蛋白浓度,应用表面增强激光解吸电离飞行时间质谱技术（SELDI-TOF-Ms）检测分枝杆菌蛋白表达,和非分枝杆菌蛋白指纹图谱比较,筛选分枝杆菌特征性蛋白。重复测定20次分枝杆菌蛋白标本,评价SELDI检测分枝杆菌蛋白分子量的重复性。结果耻垢分枝杆菌ATCC 14468有约20个蛋白峰,结核分枝杆菌ATCC 25177、土地分枝杆菌ATCC 15755、胞内分枝杆菌ATCC 13950、耻垢分枝杆菌ATCC 607有近40个蛋白峰。与非分枝杆菌蛋白指纹图谱相比,4个蛋白峰为分枝杆菌所特有。SELDI重复检测20次分枝杆菌蛋白标本显示同一蛋白峰的分子量变异系数≤0．05％。结论分枝杆菌有其特征性蛋白峰,可能有助于分枝杆菌的快速鉴定。     

双向凝胶电泳比较三种常用蛋白质提取方法

组织(或细胞)的蛋白质提取效率直接影响蛋白质双向凝胶电泳(2-DE)的分辨率.为探索建立适用于人乳腺癌细胞株MCF-7蛋白质提取的最佳条件,比较目前在双向凝胶电泳中常用的3种蛋白质提取方法对MCF-7细胞总蛋白的提取效率.MCF-7细胞经培养后,分别采用M-PER试剂、标准裂解液或含硫脲裂解液提取其总蛋白质,然后进行双向凝胶电泳,并根据凝胶上蛋白质斑点的丰度和分布特点判断所得双向电泳图谱的质量,以确定MCF-7细胞蛋白质提取的相对最佳方法.结果显示,M-PER试剂法得到的图谱分辨率较低,蛋白质主要集中分布在分子量15~70kD,pH4.7~6.3的范围内;标准裂解液法得到的图谱分辨率有所提高,蛋白质分布比M-PER试剂法得到的图谱广;硫脲裂解液法得到的图谱是三者中分辨率最高的,尤其是高丰度蛋白和高分子量蛋白分离效果比前两者好.结果表明,在3种常用的蛋白质提取方法中,硫脲裂解液对细胞蛋白质的溶解性最佳,相对更适合于提取MCF-7细胞的蛋白质,并与双向凝胶电泳条件更兼容.     

用于液质联用分析的少量卵丘颗粒细胞蛋白提取方法的比较

本研究通过对比三种常用的蛋白提取裂解液,建立适合少量卵丘颗粒细胞液质联用分析的蛋白提取方法.收集的卵细胞质内精子注入术患者的卵丘颗粒细胞,分别采用SDT、UED、RIPA裂解液提取卵丘颗粒细胞总蛋白,通过蛋白浓度测定检测蛋白提取效率,SDS-PAGE检测蛋白提取质量,并对酶解后的蛋白进行单针液质联用分析其表达谱,进而对蛋白的检测效果进行评估.蛋白浓度检测表明RIPA裂解液提取的卵丘颗粒细胞蛋白得率较UED裂解液高,蛋白凝胶条带则最为清晰,条带数量最多.液质联用检测发现UED裂解液提取的蛋白鉴定效率最高,RIPA裂解液提取的蛋白质谱峰图质量最佳,通过对鉴定蛋白亚细胞定位分析,发现RIPA裂解液对于膜蛋白鉴定效率上有明显优势,而UED裂解液可能有利于细胞核蛋白的检测.该研究表明三种方法中UED提取法更适合卵丘颗粒细胞的液质联用分析,为临床少量卵丘颗粒细胞的蛋白提取与液质联用分析提供方法依据,并为其他不易获得的少量样本的蛋白质组学提供参考.     

洋葱伯克霍尔德菌外膜蛋白双向电泳的建立与优化

目的:洋葱伯克霍尔德菌外膜蛋门的分离及双向电泳图谱的建立和优化.方法:用月桂酰基氯酸钠法提取外膜蛋白,以同相pH梯度为第一向和SDS-PAGE为第二向进行双向电泳,对裂解液成分,IPG胶条的pH和凝胶染色方法等进行优化.结果:获得外膜蛋白浓度为2.87μg/μl;最佳裂解液成分为:7mol/L尿素,2mol/L硫脲,4%Chaps,2%pharmalyte,65 mmol/L DTT,0.5%Triton X-100,10mmol/L Tris.结论:提取的外膜蛋白满足双向电泳条件;获得理想的外膜蛋白双向电泳图谱用于后续实验中.     

Analysis of differential protein expression in Acidithiobacillus ferrooxidans grown under different energy resources respectively using SELDI-ProteinChip technologies

Surface-enhanced laser desorption/ionization (SELDI)-time of flight is an affinity-based mass spectrometric method in which proteins of interest are selectively absorbed to a chemically modified surface on a chip, which allows proteomic analysis with limited material requirements. This characteristic makes it a valuable technique for microbiologists handling problematic samples, such as low cell number cultures. In this study, we explored differential-expressed proteome of Acidithiobacillus ferrooxidans cultivated with Fe(2+) and elemental sulfur separately by adopting the protein biochip SELDI approach. The cell lysates of A. ferrooxidans were applied onto Ciphergen ProteinChip WCX2, SAX2 and IMAC-Cu arrays. Proteins bound to the chips were analyzed on a ProteinChip Reader Model PBS II. A summary of the molecular masses of the differentially regulated proteins found on WCX2, IMAC-Cu and SAX2 was obtained and 28 differentially expressed proteins were found on the molecular weight range of 5.0 to 25 kDa.     

Proteomic analyzes of copper metabolism in an in vitro model of Wilson disease using surface enhanced laser desorption/ionization-time of flight-mass spectrometry

In Wilson disease, mutations in the ATP7B-gene lead to hepatic accumulation of copper that becomes toxic when the hepatic binding capacity is exceeded, leading to oxidative stress and acute liver failure. Several proteins are probably involved in dealing with the excess copper and oxidative stress. As a first step towards biomarker discovery and analyzes of copper metabolism in Wilson disease patients we characterized copper-induced changes in protein expression in cell lysates and culture media from an in vitro copper-overload model using surface enhanced laser desorption/ionization (SELDI) proteomics technology. HepG2 cells were cultured for 48 h with a physiological (0.5 microM) or a pathological (100 microM) copper concentration. Samples were applied to weak cation exchange (WCX) proteinchip arrays and chips were analyzed by time of flight (TOF)-mass spectrometry. Copper-coated IMAC chips were used to detect copper-binding proteins in cell lysate of copper depleted cells using buffers with increasing imidazole concentrations. Data from the 2 to 50 kDa range indicate that high extra-cellular copper substantially altered both intra-cellular protein expression as well as the composition of the secretome. In the lysate 15 proteins were found up-regulated, while 6 proteins were down-regulated. In culture media 21 proteins were increased while 4 proteins were decreased in abundance. Copper-coated protein chips revealed the presence of 18 high-affinity copper-binding proteins. Further identification is necessary to determine the exact cellular roles of the discovered proteins.     

Proteomic approaches to biomarker discovery in lung cancers by SELDI technology

The purpose of the present work is to identify protein profiles that could be used to discover specific biomarkers in serum and discriminate lung cancer. Thirty serum samples from patients with lung cancer (15 cases of primary brochogenic carcinoma, 9 cases of metastasis lung cancer and 6 cases of lung cancer after chemotherapy) and twelve from healthy individuals were analyzed by SELDI (Surfaced Enhanced Laser Desorption/Ionization) technology. Anion-exchange columns were used to fractionate the sera with 6 designated pH washing solutions. Two types of protein chip arrays, IMAC-Cu and WCX2, were employed. Protein chips were examined in PBSII ProteinChip Reader (Ciphergen Biosystems Inc.) and the resulting profiles between cancer and normal were analyzed with Biomarker Wizard System. In total, 15 potential lung cancer biomarkers, of which 6 were up-regulated and 9 were down-regulated, were discovered in the serum samples from patients with lung cancer. 5 of 15 these biomarkers were able to be detected on both WCX2 and IMAC-Cu protein chips. The sensitivities provided by the individual markers range from 44.8% to 93.1% and the specificities were 85.0%–94.4%. Our results suggest that serum is a capable resource for detection of lung cancer with specific biomarkers. Moreover, protein chip array system was shown to be a useful tool for identification, as well as detection of disease biomarkers in sera.     

Proteomic approaches to biomarker discovery in lung cancers by SELDI technology

Lung cancer is one of the most common tumors all over the world and one of those with higher mortality in clinic. For instance, 169500 new cases of lung cancer were estimated in the United States for 2001[1]. In recent years, both morbidity and mortality of lung cancer were reported gradually increasing in our country. Therefore, it has become an urgent task to search and discover specific biomarkers for lung cancer. In tumor genesis, certain cellular proteins must have changed their express…     

ProteinChip technology: a new and facile method for the identification and measurement of high-density lipoproteins apoA-I and apoA-II and their glycosylated products in patients with diabetes and cardiovascular disease

This paper describes a ProteinChip technology for the identification and quantification of apolipoprotein profiles in crude biological samples. Expression levels of apoA-I and apoA-II and their glycosylated products were accomplished using single 1 microL plasma samples. In the present studies, strong anionic and weak cationic exchanger ProteinChips (SAX2 and WCX2 chip surfaces) were tested, and the WCX2 chip was found to be selective for specific apolipoproteins. Using the WCX2 chip and analysis via surface-enhanced laser desorption ionization mass spectrometry (SELDI-MS), apoA-I and apoA-II were separated as sharp peaks at 28 and 17 kD and did not overlap with other serum protein peaks. Since these assays can be completed on a large number of clinical samples in approximately 1 h, further development of this technique will facilitate both epidemiological studies and therapeutic trials in assessing the role of the apolipoproteins and their glycosylated products in atherosclerosis.     

Optimization of SELDI-TOF protein profiling for analysis of cervical mucous

Cervical mucous, produced in the region where cervical neoplasia occurs, is thought to be a good choice for discovery of biomarkers to improve cervical cancer screening. In this study, SELDI-TOF MS analysis was used to evaluate parameters for protein profiling of mucous. Proteins were extracted from mucous collected with Weck-Cel^® sponges. Several parameters like extraction reagent, loading protein concentration, matrix type, bind/wash conditions and sample fractionation, on different protein chip surfaces were evaluated. SELDI peak number and consistency in the resulting spectra were used to evaluate each condition. Analysis of spectra generated by different protein chips revealed an average of 30 peaks in the 2.5–30 kDa mass range using sinnapinic acid in the unfractionated sample. Sample concentration and buffer conditions evaluated did not lead to large alterations in the profiles. Quality control spectra were reproducible with intra- and inter-assay intensity CV for CM10, H50 and Q10 arrays being less than 20% and 30% respectively. IMAC30-Cu chips had higher intra- and inter-assay CV's at 25% and 35%. Current data showed that optimizing pre-analytical parameters can help in standardization and reproducibility of protein profiles produced by cervical mucous, and thus can be used for protein biomarker discovery with the SELDI platform.     

Optimization of SELDI-TOF protein profiling for analysis of cervical mucous

Cervical mucous, produced in the region where cervical neoplasia occurs, is thought to be a good choice for discovery of biomarkers to improve cervical cancer screening. In this study, SELDI-TOF MS analysis was used to evaluate parameters for protein profiling of mucous. Proteins were extracted from mucous collected with Weck-Cel^® sponges. Several parameters like extraction reagent, loading protein concentration, matrix type, bind/wash conditions and sample fractionation, on different protein chip surfaces were evaluated. SELDI peak number and consistency in the resulting spectra were used to evaluate each condition. Analysis of spectra generated by different protein chips revealed an average of 30 peaks in the 2.5–30 kDa mass range using sinnapinic acid in the unfractionated sample. Sample concentration and buffer conditions evaluated did not lead to large alterations in the profiles. Quality control spectra were reproducible with intra- and inter-assay intensity CV for CM10, H50 and Q10 arrays being less than 20% and 30% respectively. IMAC30-Cu chips had higher intra- and inter-assay CV's at 25% and 35%. Current data showed that optimizing pre-analytical parameters can help in standardization and reproducibility of protein profiles produced by cervical mucous, and thus can be used for protein biomarker discovery with the SELDI platform.     

Proteomic analyses of arsenic-induced cell transformation with SELDI-TOF ProteinChip technology

In this study, we demonstrated that low levels (1.5 microM) of arsenite induces B[a]P-treated lung cell transformation. We then used a proteomic approach to identify protein expression by ProteinChips, which could potentially be important for transformation induced by this toxic metal. Most of the protein peaks in cell extracts of all samples, including the control, B[a]P-treated, and B[a]P + As-treated cells are identical. However, surface-enhanced laser desorption/ionization time of flight (SELDI-TOF) analysis with Cu-ProteinChips and WCX-ProteinChips revealed several dramatically different protein peaks that appeared in lung cells after being transformed by a treatment of 1.5 microM arsenite for 12 weeks. SAX2 ProteinChip also identified a prominent protein peak that was preferentially expressed in control cells. Interestingly, by using a SAX2 chip, we were able to detect several protein peaks that increased their expression in lung epithelial cells (LEC) treated with only B[a]P. Identification and characterization of these proteins may reveal the molecular basis of As-induced cell transformation and provide insight into the mechanisms by which arsenic induces carcinogenesis.     

硫酸酯酶2型基因体内表达促进化疗药物诱发的小鼠骨髓抑制恢复作用研究

采用半定量RT-PCR和重组基因体内表达法观察了硫酸酯酶2基因（Sulfatase 2,Sulf2）在5-氟脲嘧啶（5-Fluorouracil, 5-Fu）诱发的小鼠骨髓抑制和再生过程中作用。结果表明：Sulf2在小鼠骨髓抑制和再生过程中呈现先上升,后下降的动态表达;电转pcDNA3.1-Sulf2基因实验组外周血白细胞数和血小板数在5-Fu注射后第7天分别为(1216.7±457.9)/μl和(8.1±5.4)万/μl,明显低于对照组［分别为(1691.7±228.9)/μl和(14.7±2.1)万/μl］,实验组单条腿骨髓细胞总数在第7天为(94.2±21.1)万,显著低于对照组（173±59.9）万,但在第11天为(585±337.9)万,又显著地高于对照组（255±65.3）万,实验组第7天10000个骨髓细胞总集落形成数为(9±8.4),显著低于对照组（39±12.2),统计均有显著性差异（p<0.05）。这些结果提示Sulf2可能对5 Fu诱发的小鼠骨髓抑制后的再生具有促进作用。     

Search for a novel biomarker for the brain cancer astrocytoma by using surface enhanced laser desorption/ionisation (SELDI) technique.

The protein chip surface enhanced laser desorption/ionisation (SELDI) technique is a highly versatile analytical mass spectrometry system with considerable potential for detection, identification and quantitation of protein complex mixtures. Astrocytoma is a tumour of the astrocytes with a very poor prognosis. There is no effective biomarker system for detection of astrocytoma. The SELDI technique was used to study differential protein expression in astrocytoma cells in comparison to normal brain astrocytes. Several novel proteins were found to be expressed in the astrocytoma cells, not present in the astrocytes.