夹心法免疫层析试条的数学模型与仿真研究

基于夹心法免疫层析试条检测原理,结合对流扩散方程和流体动力学方程,建立了夹心法免疫层析试条动态反应过程的数学模型,并通过COMSOL软件对试条动态反应过程进行仿真.分别探究了目标待测物A浓度在0 ～ 20 mol/L,标记物P浓度在1×10-2～1×103 mol/L以及硝酸纤维素膜的孔隙率在0～1范围内变化时,检测线上夹心复合物浓度关于位置和时间的浓度变化情况,并分析了各物质初始浓度以及试条结构对于检测结果和检测时间的影响.结果表明,在一定浓度范围内,目标待测物A以及标记物P浓度的增加将提高试条的定量检测性能,而孔隙率通过影响混合液流速和混合液中各物质反应接触情况来影响检测结果.     

快速诊断疟疾的免疫层析试条的研制

开发成功了一种能快速、灵敏、高特异性检测疟疾的免疫层析试条。选自恶性疟原虫富组蛋白Ⅱ－一级结构中的九肽（ＡＨＨＡＨＨＡＡＤ），经人工合成后作为免疫原，生产了一些单表位单抗；完成了一些单抗的纯化与鉴定；制取了金标单抗并对其吸收光谱进行了分析；选取了包被单抗和金标单抗间的配对；比较了影响检测的各种因子。当用此试条检测６２名已用常规血间检法确证患有疟疾个体的全血，准确率达９３．５４％。     

快速检测甲胎蛋白的免疫层析试条的研制

研制了可简便、快速检出原发性肝癌标志物－－人血清中甲胎蛋白（AFP）的免疫层析试条。为此，研究了用国产试剂和材料制备胶体金、用此胶体金标记抗AFP单抗的影响因素以及抗AFP抗体固化条件、抗AFP抗体与其AFP结合能力等。结果表明，自制国产胶体金质量不亚于进口商品；金标单抗和固化抗体活性稳定，能分别显示出结合AFP分子不同表位的特异性。所得检测试条的检出速度在5至20min内，检测阳性阈值定为20ng AFP/mL血清。     

竞争法免疫层析试条的数学模型与仿真研究

根据竞争法免疫层析试条的检测原理,本研究将其分为TwA和TnA两种模式,结合对流扩散方程分别建立其数学模型,并运用COMSOL软件对试条的动态反应过程进行仿真,得到检测线和质控线上各复合物浓度关于各影响因素的关系曲线.在TwA模式中,分析了待测物浓度[A0]=0~20 mol/L,标记物浓度[P0]=0.01~100 mol/L,检测线位于5~20 mm位置等因素对于检测结果的影响;在TnA模式中,分析了[A0]=0~20 mol/L, [P0]=0.01~100 mol/L, [A0]和[P0]两种物质浓度及孔隙率等因素对于检测结果的影响.结果表明,本研究建立的竞争法模型与仿真能探究各参数对于检测结果的影响,优化试条性能,从而提高试条检测灵敏度和实现定量检测.     

磁固相萃取与胶体金免疫层析试纸条联用检测食品中氯霉素

本文建立了磁固相萃取前处理与胶体金免疫层析试纸条联用检测食品中氯霉素(CAP)的分析方法。蜂蜜和鸡蛋样品经磁固相萃取后,再用检测牛奶样品中CAP的胶体金免疫层析试纸条检测。结果表明:两者联用后使得只能用于检测牛奶样品中CAP的试纸条也能应用于蜂蜜和鸡蛋等样品,而且方法的检出限在蜂蜜和鸡蛋样品中低至0.2ng/g。该联用方法扩大了CAP试纸条的应用范围,同时降低了检测成本。     

氟苯尼考胶体金免疫层析定量检测方法的建立

建立了定量检测氟苯尼考的胶体金免疫层析方法.对胶体金标记抗体时溶液pH和抗体浓度、金标抗体用量、检测线上抗原浓度以及检测时间进行了优化.采用胶体金试纸条读取仪测定试纸条检测线和质控线的信号强度,以标准品的浓度为横坐标,阳性样本和阴性样本的检测线/质控线的信号比值(Bx/B0)为纵坐标建立标准曲线.结果表明,胶体金免疫层析试纸定量检测氟苯尼考的线性范围为0.1~1.5 ng/mL,检出限为0.08 ng/mL,检测时间为15 min.本方法具有简便、快速和可定量等特点,适于大批量样品的现场筛查.     

五氯酚免疫层析检测试纸条的研究

利用胶体金免疫层析技术建立了一种快速检测五氯酚(PCP)残留的方法。采用柠檬酸三钠还原法制备大小一致、分布均匀、粒径为20 nm的胶体金颗粒,以此标记五氯酚抗体,制备金标抗体。将五氯酚包被抗原和羊抗鼠二抗分别结合于硝酸纤维膜上,依次将型号Millipore135硝酸纤维膜、型号VL78金标垫、型号SB06样品垫及吸水纸组装于PVC底板上,组装成胶体金免疫层析检测试纸条。通过试纸条上颜色的深浅,检测样品中PCP的残留量。试纸条检出限为10 ng/mL,检测时间为5 min。该方法检测所需试剂已预先包被在试纸条上,操作简单、重复性好、成本低廉,可用于五氯酚的现场快速检测。     

水样中左旋18-甲基炔诺酮的胶体金免疫层析试剂条的研制

研制了一种检测水样中左旋18-甲基炔诺酮(LNG)含量的胶体金免疫层析试剂条.基于包被抗原和检测物对金标抗体的竞争反应,通过可目测的胶体金标记物而得到直观的检测结果.试剂条对LNG的检测,灵敏度为10 ng·ml-1,在10min内显示结果;与己烯雌酚、雌三醇,17(-雌二醇,17β-雌二醇、雌酮、甲泼尼龙、泼尼松龙和...     

菊酯类农药广谱型免疫层析试纸条的研究及应用

建立了菊酯类农药广谱型免疫层析检测方法,可同时检测水果、蔬菜中12种甲氰菊酯、溴氰菊酯、氯氰菊酯、三氟氯氰菊酯农药残留。以粒径20 nm的胶体金标记羊抗小鼠IgG抗体于金标垫上,分别固定包被原(检测线,T线)、兔抗山羊 IgG 抗体(质控线, C 线)于硝酸纤维素膜( NC 膜)上,与吸水垫及聚氯乙烯( PVC)底板组合成层析试纸条。10 g样品经乙腈提取,PBS稀释4倍,取100μL与菊酯类农药的单克隆抗体混合后,直接用于试纸条检测。结果表明,试纸条对甲氰菊酯、溴氰菊酯、氯氰菊酯、三氟氯氰菊酯农药的裸眼观察检测灵敏度为0.5,5.0,5.0和5.0μg/mL,检测时长为8~10 min,采用QuEChERS方法,方法检测灵敏度可提高16倍。对蔬菜和水果的方法验证表明,除辣椒基质干扰呈假阳性外,其它样本的检测结果均与GC方法结果一致。试纸条采用金标羊抗小鼠IgG二抗的方法,使检测结果的重现性更好、更稳定,且抗基质干扰能力强,为菊酯类农药的累积毒性检测提供了新方法。     

基于免疫磁分离的荧光微球免疫层析法检测猪霍乱沙门氏菌

建立了基于免疫磁分离的荧光微球免疫层析法,检测猪霍乱沙门氏菌.待检样品经免疫磁分离富集和热洗脱处理后,用荧光微球免疫层析试纸条进行检测.每毫克纳米磁珠标记30μg抗体制备的免疫磁珠,对浓度为102 ～ 106 CFU/mL的猪霍乱沙门氏菌的捕获率均大于90％,特异性好;在pH=6时,以300μ,g/mg猪霍乱沙门氏菌单抗11D8-D4标记荧光微球,制备免疫荧光微球;以2.0 mg/mL猪霍乱沙门氏菌单抗5F11-B11喷涂检测线(T线),以1.0 mg/mL驴抗鼠IgG喷涂质控线(C线),制备免疫层析试纸条.采用建立的基于免疫磁分离的荧光微球免疫层析方法检测猪霍乱沙门氏菌,在PBS缓冲液中检出限为1.5×105 CFU/mL,牛奶中检出限为7.6×105 CFU/mL,与直接采用荧光微球免疫层析方法检测相比,检出限分别降低了10倍和200倍.本方法可有效富集牛奶中的沙门氏菌,避免了基质干扰,灵敏度大大提高,具有较好的应用前景.     

基于免疫胶体金试纸条检测盐酸克伦特罗的便携式光电型传感器

利用免疫竞争抗制原理制备检测盐酸克伦特罗的免疫纳米金试纸条,盐酸克伦特罗与CLB-BSA复合物竞争性结合胶体金上抗体的有限位点,从而使试纸条上的检测带显色减弱或消失.将显色后的试纸条插入自行研制的光电型传感器的测试孔内,根据反射光的强弱计算出克伦特罗的浓度.结果表明:用光电传感方法检测盐酸克伦特罗的线性范围为1～10 μg/L,检出限为0.05 μg/L,回收率为85.5％～96.0％.此光电型传感器检测克伦特罗具有简便、快速、灵敏、特异性强的优点.     

免疫胶体金技术的应用与展望

免疫胶体金技术是一种新型固相标记免疫检测技术,因其独特的性质在许多领域得到广泛应用和快速发展。简述了免疫胶体金技术在电镜、光镜快速检测诊断中的发展以及在生物医学、免疫组织化学和细胞生物学等领域的研究和应用。未来免疫胶体金技术在提高胶体金制备质量的同时将实现定量和多元化检测。     

Colloidal woodpile structure: three-dimensional photonic crystal with a dual periodicity

With planar photolithography and self-assembly techniques, multilayer colloidal crystals with a woodpile structure were fabricated. They represent a new kind of photonic crystals, that is, three-dimensional (3D) photonic crystals with a dual periodicity; one comes from the face-centered cubic (fcc) structure within the colloidal crystal strips and the other one results from the periodic arrangement of the colloidal crystal strips.     

Studies on the interaction of colloidal gold and serum albumins by spectral methods

The interactions of colloidal gold and serum albumins, including bovine serum albumin (BSA) and human serum albumin (HSA), were studied by fluorescence and absorption spectrometry. Fluorescence quenching spectrometry was applied to study the interactions between colloidal gold and serum albumins. At pH 7.4 phosphate-buffered saline (PBS), the intensity of fluorescence emission spectrum of serum albumins decreased in the presence of colloidal gold, which indicated that colloidal gold quenched the fluorescence of serum albumins. Experimental results indicated that the combination reactions of colloidal gold and serum albumins were static quenching processes. Based on the effect of colloidal gold on fluorescence intensity, the binding constants, the numbers of binding sites and the acting forces between colloidal gold and serum albumins were found.     

A novel enhancement assay for immunochromatographic test strips using gold nanoparticles

The immunochromatographic assay is a well-known and convenient diagnostic system. In this report, the development of a novel enhancement assay for the test strips is described. Additionally, this highly sensitive immunochromatographic assay was applied to detect human chorionic gonadotropin hormone (HCG) as the model case. The primary antibody-conjugated gold nanoparticles were used as the enhancer of the standard method. The primary antibodies were immobilized within a defined detection zone (test line) on the diagnostic nitrocellulose membrane. The secondary antibodies were conjugated with colloidal gold nanoparticles. In combination with an effective sample pretreatment, the gold-conjugated antibodies and the primary antibodies formed a sandwich complex with the target protein. Within the test line, the sandwich complex was immobilized, and furthermore, concentrated by the enhancer resulting in a localized surface plasmon resonance (LSPR) phenomenon and a distinct red color on the test line. The intensity of color of the red test line (signal intensity), which correlated directly with the concentration of the target protein in the standard or spiked samples, was assessed visually and by computer image analysis using a three-determination analysis. Under optimum conditions, the limit of detection (LOD) for HCG assay was 1 pg/mL. When using human serum, 10 pg/mL of HCG could be detected. We have also spiked total prostate-specific antigen (TPSA) in female serum. The LOD for TPSA was determined as 0.2 ng/mL. With this method, the quantitative determination of the target protein could be completed in less than 15 min. Our novel immunochromatographic strips using the enhancing method based on LSPR of gold nanoparticles are useful as a rapid and simple screening method for the detection of important analytes for medical applications, environmental monitoring, food control, and biosecurity.      

Solution-based direct readout surface enhanced Raman spectroscopic (SERS) detection of ultra-low levels of thiram with dogbone shaped gold nanoparticles

We report the use of two different sizes of dogbone shaped gold nanoparticles as colloidal substrates for surface enhanced Raman spectroscopy (SERS) based detection of ultra-low levels of thiram, a dithiocarbamate fungicide. We demonstrate the ability to use a solution based, direct readout SERS method as a quantitative tool for the detection of ultra-low levels of thiram. The two different sizes of dogbone shaped gold nanoparticles are synthesized by using the seed-mediated growth method and characterized by using UV-visible spectroscopy and transmission electron microscopy (TEM). The smaller dogbone shaped nanoparticles have an average size of 43 ± 13 nm. The larger dogbone shaped gold nanoparticles have an average size of 65 ± 15 nm. The nanoparticle concentration is 1.25 × 10(11) nanoparticles per mL for the smaller dogbone shaped gold nanoparticles and is 1.13 × 10(11) nanoparticles per mL for the larger dogbone shaped gold nanoparticles. Different concentrations of thiram are allowed to bind to the two different sizes of dogbone shaped gold nanoparticles and the SERS spectra are obtained. From the calibration curve, the limit of detection for thiram is 43.9 ± 6.2 nM when the smaller dogbone shaped gold nanoparticles are used as colloidal SERS substrates In the case of the larger dogbone shaped gold nanoparticles, the limit of detection for thiram is 11.8 ± 3.2 nM. The lower limit of detection obtained by using the larger dogbone shaped gold nanoparticles as colloidal substrates is due to the lightning rod effect, higher contributions from the electromagnetic enhancement effect, and larger number of surface sites for thiram to bind.     

Investigation on the interaction between colloidal gold and human complement factor 4 at different pH by spectral methods

The interaction between colloidal gold and human complement factor 4 (human C4) at different pH was investigated by spectral methods, including absorption and resonance light-scattering spectrometry. According to the changes of color and absorption spectra of colloidal gold solution in presence of human C4, the interaction between colloidal gold and human C4 was quantitatively investigated using a semi-empirical "flocculation parameter". At the same time, the changes of resonance light-scattering spectra and transmission electron microscopy (TEM) images indicate that the aggregation of colloidal gold happens by electrostatic interaction in presence of human C4 in the pH range 5-6. However, the colloidal gold solution remains stable at pH >6 and pH <5 due to the repulsive electrostatic interaction between colloidal gold and human C4. The flocculation parameter is directly proportional to the concentration of human C4 in the range from 9.7 to 233.0 microgl(-1). In addition, the interactions between the colloidal gold and bovine serum albumin (BSA) as well as human serum albumin (HSA) were also investigated using the same methods. It was found that there was no aggregation of colloidal gold in presence of BSA and HSA in the pH range 5-6. However, when the pH of solution is 4, the aggregation of colloidal gold happens. Because BSA and HSA have different structure, the intensity of aggregation of colloidal gold in presence of BSA is greater than that in presence of HSA at pH 4.     

Reveal for Salmonella test system.

The Reveal for Salmonella (RSS) test system is a presumptive qualitative test that detects the presence of Salmonella organisms in foods within 21 h total testing time, allowing the user to release negative products 24 h earlier than when using other rapid test kits. Foods are enriched with a proprietary resuscitation medium called Revive and then selectively enriched with either Selenite Cystine or Rappaport-Vassiliadis selective media. The enriched culture is used to inoculate the RSS detection device, which initiates a lateral flow through a reagent zone containing anti-Salmonella antibodies conjugated to colloidal gold particles that capture antigens present in the culture. The antigen-antibody complex migrates farther and is captured by an additional anti-Salmonella antibody, causing the colloidal gold to precipitate and form a visual line, indicating a positive result. A procedural control line also will form regardless of the presence of Salmonella organisms to indicate the test is working properly. Existing AOAC Official Methods for Salmonella organisms require a 48 h enrichment before testing. Hence, a food product has to be held before release, adding extra cost to the company and the consumer. The RSS test system was evaluated by quantitative spiking studies. Although AOAC encourages inclusion of naturally contaminated foods, almost all microbiological AOAC validation studies have been performed with artificially contaminated foods for absolute control over the study. The RSS test system is designed to test many food types for Salmonella organisms and has a limit of detection of 5-10 colony-forming units (cfu)/25 g with a false-negative rate of < 1% and a false-positive rate of < 5.0%. It showed an 81% overall agreement with the traditional procedure of the U.S. Department of Agriculture's Food Safety Inspection Service.     

Study on the Interaction of Colloidal Gold with Taq DNA Polymerase

The interaction of colloidal gold with Taq DNA polymerase （Taq） was investigated in this study. Taq-gold conjugate was formed by adding the enzyme to the colloidal gold solution, as evidenced by UV-Vis spectroscopy, X-ray photoelectron spectroscopy, and photon cross correlation spectroscopy measurements. The conjugate was further characterized by transmission electron microscopy. It was found that the Taq-gold conjugate particles were still spherical and well-dispersed. The influence of gold nanoparticles on the bioactivity of Taq was studied by analyzing the yield of the polymerase chain reaction amplification. Results indicated that the enzymatic activity of Taq decreased after interaction with the colloidal gold.