乙酸胁迫酵母细胞凋亡过程中单个线粒体损伤的拉曼光谱分析

应用激光光镊拉曼光谱技术(LTRS)作为一种非入侵分析线粒体的工具,结合氧电极法、紫外分光光度计法,研究乙酸胁迫酵母细胞后提取的线粒体,以及直接胁迫正常酵母细胞的离体线粒体的拉曼光谱.结果显示,乙酸胁迫酵母细胞后提取的线粒体的拉曼光谱,归属于核酸的谱峰(1081和1301 cm-1)、蛋白质的谱峰(872,1445,1604和1657 cm-1)、脂类的谱峰(1125,1301,1445和1657 cm-1)、Cyt c的特征峰(750和1125 cm-1)、线粒体呼吸特征峰(1604 cm-1),都随着诱导程度的加深而降低,与常规法测定的指标呼吸率,磷氧比,细胞色素C含量的降低,MDA含量的升高的变化趋势相似;乙酸直接胁迫线粒体的拉曼光谱,归属于核酸的谱峰(1081和1301 cm-1),蛋白质的谱峰(872,1445,1604和1657 cm-1),脂类的谱峰(1125,1301,1445和1657 cm-1),Cyt c的特征峰(750和1125 cm-1),线粒体呼吸特征峰(1604 cm-1),都随着诱导程度的加深而降低,与常规法测定的指标呼吸率、磷氧比、细胞色素C含量的降低,MDA含量的升高的变化趋势相似.结果表明,乙酸胁迫细胞过程中,乙酸进到细胞内可能直接作用于线粒体,引起线粒体内物质的释放,导致依赖于线粒体途径的细胞凋亡.     

激光拉曼光谱内标法直接测定甲醇含量

<正>激光拉曼光谱法作为一种新型无损检测技术,广泛应用于样品的定性、定量分析[1-3]。目前,样品中甲醇的定量分析方法常用的有气相色谱法[4]、分光光度法[5]和传感器法[6]等。本工作通过不同浓度的甲醇拉曼光谱特征峰(1 016.46cm-1)与乙醇的拉曼光谱特征峰(877.95cm-1)组成相对强度比,建立线性回归方程。本法具有测定简单、操作方便,无需添加其他化学试剂,可用于甲醇含量的直接检测。     

软骨细胞体外增殖去分化的拉曼光谱分析

基于显微拉曼光谱技术,对组织工程的软骨种子细胞在传代增殖过程中的去分化进行单细胞分析。首先,对体外单层培养的第1-4代(P1-P4)大鼠软骨细胞样本进行了单细胞拉曼光谱检测,由此识别出软骨细胞中各种碱基、糖基、氨基酸等主要物质分子结构的特征峰集合。随后,分析拉曼光谱中若干重点特征峰强度随细胞传代次数的变化,发现软骨细胞体外增殖过程中核酸(789、1094、1576 cm~(-1))含量降低、Ⅱ型胶原(特异组分为羟脯氨酸,1207 cm~(-1))和蛋白聚糖(特异组分为糖胺聚糖,1042、1063、1126、1160 cm~(-1))合成下降、脂质(1304 cm~(-1))及磷酸盐(957 cm~(-1))含量增加等分子水平变化,从而在活体单细胞层次初步揭示了去分化引起软骨细胞增殖变缓、分泌减弱、形态纤维化等现象的分子机制。     

活体小鼠中单个红细胞的拉曼光谱分析

应用拉曼光谱与光镊技术对活体小鼠毛细动脉和静脉血管中的全血以及毛细血管中的红细胞和体外的全血及单个红细胞进行研究;光谱分析显示,可以获得活体血液的拉曼光谱;在动脉毛细管和静脉毛细管中可以观察到清晰的携氧与去氧血液的不同光谱;体内血管中血红细胞的血红蛋白浓度比体外的更高,在动脉毛细管中的血红细胞的携氧态特征峰明显,且具有...     

激光拉曼光谱内标法直接测定甲醇浓度

利用甲醇溶液中的CH3对称伸缩峰(2843 cm-1)的激光拉曼光谱峰,同时以本底溶液水为内标物,组成相对强度,对溶液中的甲醇含量进行了测定研究,建立了激光拉曼光谱直接法测定甲醇含量的方法,其线性范围为5%~40%,线性相关系数为0.9966,检出限为0.29%。并对模拟样品和制备液相色谱待回收废液进行了甲醇浓度的测定,其浓度分别为13.7%、9.41%和58.8%,RSD分别为0.78%、0.75%和1.34%。该方法简单、操作方便,无需添加其它任何化学试剂等优点。     

拉曼光谱法定量分析焦磷酸根离子的含量

应用拉曼光谱技术研究了焦磷酸钾、硝酸钾、磷酸二氢钾、乙二胺四乙酸钠等十余种可溶性盐水溶液以及它们的混合物溶液的拉曼光谱特征,考察了共存组分对焦磷酸根拉曼光谱特征峰的影响;建立了基于拉曼光谱技术定量分析溶液中焦磷酸根离子含量的方法。结果表明,以硝酸钾为内标物,保持被测溶液pH 11,焦磷酸根离子拉曼光谱特征峰强度与硝酸根离子拉曼光谱特征峰强度之比值对焦磷酸根浓度呈良好的线性关系,所得线性回归方程为y=1.2110x+0.1515,相关系数R2=0.9996;已经研究过的十余种可溶性盐共存物几乎不干扰焦磷酸根离子的定量分析。     

激光拉曼光谱内标法直接测定乙醇浓度

采用激光拉曼光谱对醇类样品中的乙醇含量进行直接测定。通过不同浓度乙醇的拉曼光谱特征峰(CCO面内伸缩振动884cm-1)与本底水峰组成相对强度比,建立线性回归方程,结果表明,线性范围为4%~40%,线性相关系数为0.9975;检出限为1.02%;回收率为82.0%~105.0%。对白酒、清酒、杨梅酒和医用酒精棉进行了测定,其乙醇平均浓度分别为36.1%、15.5%、23.7%和79.1%;RSD分别为0.22%、1.75%、2.49%和2.76%。此方法具有快速、简便、直接、绿色、对样品无损等优点,适用于白酒类、医用酒精等乙醇含量的检测。     

拉曼镊子在生物单细胞中的应用与进展

拉曼镊子(Raman tweezers)是将激光光镊(Optical tweezers)与显微拉曼光谱(Raman spectroscopy)结合的光学技术,可以在接近自然状态下研究单个生物细胞或细胞器.因其有无直接接触、无损伤、快速识别、实时追踪等特点,广泛用于生物细胞的识别、探测、筛选等.研究显示,拉曼镊子在微观生物研究的应用中,可提高拉曼光谱的信噪比,也能实现生化动力学过程的实时跟踪,从而能深刻了解细胞内生物大分子的活动规律.本文着重介绍了拉曼镊子的起源、原理及其在单细胞中的应用以及展望.     

快速线扫描拉曼成像技术在研究CaSki细胞凋亡过程中的应用

应用快速线扫描拉曼成像技术研究了在抗肿瘤药物顺铂诱导下宫颈癌Ca Ski细胞凋亡过程中细胞色素c、蛋白质和脂质等的时空变化规律.结果表明,细胞色素c与蛋白质的相对拉曼峰强可以反映细胞凋亡程度.与常用的表征细胞活性的噻唑蓝(MTT)实验的统计方法相比,利用拉曼成像技术可以更灵敏地观察到细胞凋亡早期生物活性分子的变化,从而在单细胞水平检测细胞凋亡过程,为解析药物与细胞的作用机制提供分子水平信息.     

异硫氰基孔雀石绿受激拉曼光谱研究

本文报道了具有时间分辨能力的全频宽带受激拉曼（BBSRS）系统和关于异硫氰基孔雀石绿（MGITC）受激拉曼光谱（sRs）的研究．BBSRS系统的探测光为450-800nm宽带连续白光,泵浦光为280～900nm范围内连续可调谐的ps窄带可见光（带宽≈7．5cm-1,脉宽≈2．5ps）．在合适的泵浦波长下,该系统可同时获取拉曼损失和拉曼增益光谱．MGITC的SRS研究结果表明,当拉曼损失谱峰出现在最大吸收波长（≈627nm）时,共振SRS谱峰强度最大;当泵浦或增益谱峰在最大吸收波长附近时,未观察到明显的共振拉曼信号;共振峰强度随浓度增大而增大,随泵浦功率增大而迅速增大,后趋于饱和;共振和非共振峰强在延时零点附近达到最大值,并随延时绝对值的增大而减小．     

Optical tweezers for medical diagnostics

Laser trapping by optical tweezers makes possible the spectroscopic analysis of single cells. Use of optical tweezers in conjunction with Raman spectroscopy has allowed cells to be identified as either healthy or cancerous. This combined technique is known as laser tweezers Raman spectroscopy (LTRS), or Raman tweezers. The Raman spectra of cells are complex, since the technique probes nucleic acids, proteins, and lipids; but statistical analysis of these spectra makes possible differentiation of different classes of cells. In this article the recent development of LTRS is described along with two illustrative examples for potential application in cancer diagnostics. Techniques to expand the uses of LTRS and to improve the speed of LTRS are also suggested.     

An integrated optofluidic platform for Raman-activated cell sorting

We report on integrated optofluidic Raman-activated cell sorting (RACS) platforms that combine multichannel microfluidic devices and laser tweezers Raman spectroscopy (LTRS) for delivery, identification, and simultaneous sorting of individual cells. The system allows label-free cell identification based on Raman spectroscopy and automated continuous cell sorting. Two optofluidic designs using hydrodynamic focusing and pinch-flow fractionation are evaluated based on their sorting design and flow velocity effect on the laser trapping efficiency at different laser power levels. A proof-of-principle demonstration of the integrated optofluidic LTRS system for the identification and sorting of two leukemia cell lines is presented. This functional prototype lays the foundation for the development of a label-free cell sorting platform based on intrinsic Raman markers for automated sampling and sorting of a large number of individual cells in solution.     

Ce1-xGdxO2-δ固溶体中缺陷物种的拉曼光谱研究

采用溶胶-凝胶法制备一系列Ce1-xGdxO2-δ固溶体。利用紫外(325 nm)和可见(514 nm)Raman光谱,X射线粉末衍射(XRD),透射电子显微镜(TEM)和紫外可见漫反射光谱(UV-Vis DRS),考察了Ce1-xGdxO2-δ固溶体的缺陷物种的分布以及Gd含量对缺陷浓度的影响。结果表明:Ce1-xGdxO2-δ固溶体中存在氧缺位(～560 cm-1)和GdO8型缺陷结构(～600 cm-1)。根据样品对Raman激发光的吸收,紫外Raman光谱反映样品的表层信息,可见Raman光谱反映样品的整体信息。Ce1-xGdxO2-δ固溶体表层氧缺位(να)和GdO8型缺陷物种的浓度(νβ)均高于固溶体体相,这归因于缺陷物种的表面富集。然而,相比于GdO8型缺陷物种,体相中氧缺位浓度增加较表层中的更显著。     

金黄色葡萄球菌及其甲氧苯青霉素耐药性的MALDI-TOF MS鉴定

用MALDI－TOS MS细菌指纹图谱鉴定细菌，建立区分金黄色葡萄球菌甲氧苯青霉素耐药株和敏感株的MALDI－TOF MS分析方法，检测了76株从临床标本中分离得到的金黄色葡萄球菌，用软件进行聚类分析，以nuc(耐热核酸酶）基因和mecA(耐药）基因聚合酶链反应（PCR）检测结果为参照，74％的菌株经MALDI－TOF MS给出了正确的鉴定结果；金黄色葡萄球菌甲氧苯青霉素耐药株和敏感株的质谱图有很大差别，各自有其特征峰；经过软件聚类分析，76株实验菌株划敏感群和耐药群；与PCR检测结果对照，有7株菌PCR检测mecA基因为阴性，而经MALDI－TOF MS鉴定为耐药株，表型鉴定表明其中有5株为敏感株；利用细菌指纹图谱和数据库检索对大多数菌株实现了正确鉴定；MALDI－TOF MS分辨率高，甚至可以区分株间的差异，实现了区分金黄色葡萄球菌甲氧苯青霉素耐药株和敏感株；结果表明MALDI－TOF MS提供了一个很有前景的鉴定细菌的快速方法。     

Elucidation of cell killing mechanism by comparative analysis of photoreactions on different types of bacteria

The mechanism of biocidal action of nano titania on Escherichia coli and Staphylococcus aureus has been evaluated by various biochemical techniques like lipid peroxidation, hydrolysis of orthonitrophenol β-D-galactopyranoside, estimation of protein-amino acid and bacterial nucleic acids leakage into solution, in addition to morphology studies by electron microscopy (TEM and SEM) and K(+) ion leakage by inductively coupled plasma optical emission spectrometry. The active anatase phase of nano titania has been synthesized by sol-gel and pulverization techniques to obtain particle sizes averaging around 11 nm. The nano semiconductor with a bandgap of 3.2 eV responds well to the UV source to liberate reactive oxygen species (ROS). Gram negative bacteria easily succumb to the ROS at a faster rate than gram-positive bacteria with an observable difference in the mode of attack. The use of analytical techniques revealed the release of peroxidized lipid (26 nmol mL(-1) ) and protein content (370 μg mL(-1)) with a K(+) ion concentration of 22 000 ppb on complete destruction of E. coli.     

DNA碱基激光拉曼光谱检测方法的研究

以激光拉曼光谱仪采集腺嘌呤(A)、鸟嘌呤(G)、胞嘧啶(C)、胸腺嘧啶(T)的拉曼光谱图,分析了各碱基谱峰归属,并依据归属结果检测混合碱基组成。结果显示:4种碱基的特征峰集中在175～1 800cm~(-1)。相同积分时间和激光功率条件下,该波段内嘌呤碱基的激光拉曼光谱峰高于嘧啶碱基的谱峰。腺嘌呤、鸟嘌呤、胞嘧啶、胸腺嘧啶分别在723、648、791、1 368 cm~(-1)处的谱峰最强,利用这些特征峰能在2min内鉴别出混合碱基中的各碱基。     

呼吸内科下呼吸道感染细菌分布及其耐药性分析

目的探析呼吸内科下呼吸道感染细菌分布及其耐药性。方法选择湖北省孝感市中心医院呼吸内科收治1 537例下呼吸道感染患者,行痰液培养明确细菌分布并进行药敏试验掌握抗菌药物耐药情况。结果 1 537例患者共得到672份(43.72%)阳性标本,所获得菌株共782例,其中546例(69.82%)为革兰阴性球菌、157(20.08%)为革兰阳性球菌、79例(10.10%)为真菌。金黄色葡萄球菌、表皮葡萄球菌、肺炎链球菌主要对万古霉素、呋喃妥因、亚胺培南等有较高耐药性。结论革兰阴性球菌为下呼吸道感染最常见病原菌,包括铜绿假单胞菌、鲍式不动杆菌等,耐药分析显示金黄色葡萄球菌、表皮葡萄球菌、肺炎链球菌主要对万古霉素、呋喃妥因、亚胺培南、左氧氟沙星等耐药性高,临床用药时需予以注意。     

Electronic and resonance Raman spectra of [Au2(CS3)2]2-. Spectroscopic properties of a "short" Au(I)-Au(I) bond

The anion [Au2(CS3)2]2- has an unusually short Au-Au distance (2.80 A) for a binuclear Au(I) complex. We report detailed Raman studies of the nBu4N+ salt of this complex, including FT-Raman of the solid and UV/vis resonance Raman of dimethyl sulfoxide solutions. All five totally symmetric vibrations of the anion have been located and assigned. A band at delta nu = 125 cm-1 is assigned to nu (Au2). The visible-region electronic absorption bands (384 (epsilon 30,680) and 472 nm (epsilon 610 M-1 cm-1)) are attributable to CS3(2-) localized transitions, as confirmed by the dominance of nu sym(C-Sexo) (delta nu = 951 cm-1) in RR spectra measured in this region. An absorption band at 314 nm (22,250 M-1 cm-1) is assigned as the metal-metal 1(d sigma*-->p sigma) transition, largely because nu sym(C-Sexo) is not strongly enhanced in RR involving this band. Observation of the expected strong resonance enhancement of nu (Au2) was precluded as a result of masking by intense solvent Rayleigh scattering in the UV.     

Determination of nucleic acids based on shifting the association equilibrium between tetrasulfonated aluminium phthalocyanine and acridine orange

Based on the ability of nucleic acids to shift the association equilibrium of the ion-association complex of Acridine Orange and tetrasulfonated aluminium phthalocyanine, thus leading to an increase in the phthalocyanine fluorescence, a method is suggested for the fluorimetric determination of nucleic acids. Investigations were carried out on the spectral characteristics, order of addition of reagents, selection of the buffer system, effect of pH, influence of reaction time, effect of salt, the usage of reagents, interference of foreign substances and the effect of different acridine derivatives. Under the optimum conditions, the calibration graphs for the determination of calf thymus DNA (CT DNA), salmon DNA (SM DNA) and yeast RNA were linear over the ranges 0.04-1.2, 0.04-1.2 and 0.1-1.2 micrograms cm-1, respectively. The detection limits for CT DNA, SM DNA and RNA were 17, 24 and 98 micrograms cm-3, respectively. The relative standard deviation (n = 6) was within 4.6% for the detection of samples. The method was applied to the determination of Staphylococcus aureus DNA and the result was in agreement with that achieved by a UV method.     

Rapid detection of Staphylococcus aureus by a combination of monoclonal antibody-coated latex and capillary electrophoresis

The rapid detection of pathogenic bacteria is extremely important in biotechnology and clinical diagnosis. CE has been utilized in the field of bacterial analysis for many years, but to some extent, simultaneous separation and identification of certain microbes from complex samples by CE coupled with UV detector is still a challenge. In this paper, we propose a new strategy for rapid separation and identification of Staphylococcus aureus (S. aureus) in bacterial mixtures by means of specific mAb-coated latex coupled with CZE. An appropriate set of conditions that selectively isolated S. aureus from the microorganisms Escherichia coli, Pseudomonas aeruginosa, and Klebsiella pneumoniae were established. S. aureus could be differentiated from the others by unique peaks in the electropherograms. The validity was also confirmed by LIF with antibodies specific to both the latex and the microbial cells. The LOD is as low as 9.0 x 10(5) colony forming unit/mL. We have also utilized this technology to identify S. aureus in a stool sample coming from a healthy volunteer spiked successfully with S. aureus. This CZE-UV technique can be applied to rapid diagnosis of enteritis caused by S. aureus or other bacterial control-related fields needing rapid identification of target pathogens from microbial mixtures. In theory, this method is suitable for the detection of any bacterium as long as corresponding bacterium-specific antibody-coated latex is available.