INVESTIGATION OF LIPOSOME BASED IMMUNOMIGRATION SENSORS FOR THE DETECTION OF POLYCHLORINATED-BIPHENYLS

被引：63

作者：

ROBERTS, MA ^{[1
]}

DURST, RA ^{[1
]}

机构：

[1] CORNELL UNIV,INST COMPARAT & ENVIRONM TOXICOL,GENEVA,NY 14456

来源：

ANALYTICAL CHEMISTRY | 1995年 / 67卷 / 03期

关键词：

D O I：

10.1021/ac00099a002

中图分类号：

O65 [分析化学];

学科分类号：

070302 ; 081704 ;

摘要：

The use of immunospecific Liposome migration offers many advantages for the extralaboratory detection of environmental contaminants. Devices utilizing this technique are fast, easy to use, and robust and respond to the presence of analyte at low-parts-per-billion concentrations, Investigations have been carried out that determine optimal interactions for key components of these assays, and techniques are presented for the development of generalized liposome immunoassays. Two complementary prototype liposome-based immunomigration techniques have been developed for the detection of polychlorinated biphenyls (PCBs). The liposome immunocompetition assay format measures the competitive reaction between analyte-tagged liposomes and the sample analyte for immobilized antibodies and can detect 0.4 nmol of PCB in less than 8 min. A more sensitive format, the liposome immunoaggregation (LIA) assay detects the inhibition of immunospecific liposome aggregation in solution and can detect 2.6 pmol of PCB in less than 23 min. Laser diffraction particle sizing has been used to study LIA-induced increases in liposome size over time and to determine optimal conditions for the application of this technique. Both formats utilize capillary action to transport liposome-containing solutions along strips of nitrocellulose. Measurement of color intensity is then carried out visually or with a desktop scanner.

引用

页码：482 / 491

页数：10

共 41 条

[1]

ALLEN MP, 1990, CLIN CHEM, V36, P1591

[2] SCREENING FOR DRUGS OF ABUSE WITH THE ROCHE ONTRAK ASSAYS [J].

ARMBRUSTER, DA ;

KROLAK, JM .

JOURNAL OF ANALYTICAL TOXICOLOGY, 1992, 16 (03) :172-175

[3] CONTACT-DEPENDENT, IMMUNECOMPLEX-MEDIATED LYSIS OF HAPTEN-SENSITIZED LIPOSOMES [J].

BABBITT, B ;

BURTIS, L ;

DENTINGER, P ;

CONSTANTINIDES, P ;

HILLIS, L ;

MCGIRL, B ;

HUANG, L .

BIOCONJUGATE CHEMISTRY, 1993, 4 (03) :199-205

[4] THE USE OF TWEEN-20 AS A BLOCKING-AGENT IN THE IMMUNOLOGICAL DETECTION OF PROTEINS TRANSFERRED TO NITROCELLULOSE MEMBRANES [J].

BATTEIGER, B ;

NEWHALL, WJ ;

JONES, RB .

JOURNAL OF IMMUNOLOGICAL METHODS, 1982, 55 (03) :297-307

[5]

Brown WR, 1991, IMMUNOCHEMISTRY SOLI, P151

[6] HIGHER-ORDER SELF-ASSEMBLY OF VESICLES BY SITE-SPECIFIC BINDING [J].

CHIRUVOLU, S ;

WALKER, S ;

ISRAELACHVILI, J ;

SCHMITT, FJ ;

LECKBAND, D ;

ZASADZINSKI, JA .

SCIENCE, 1994, 264 (5166) :1753-1756

[7] MICROPARTICLE-ENHANCED NEPHELOMETRIC IMMUNOASSAY .1. MEASUREMENT OF ALPHA-S-CASEIN AND KAPPA-CASEIN [J].

COLLARDBOVY, C ;

MARCHAL, E ;

HUMBERT, G ;

LINDEN, G ;

MONTAGNE, P ;

ELBARI, N ;

DUHEILLE, J ;

VARCIN, P .

JOURNAL OF DAIRY SCIENCE, 1991, 74 (11) :3695-3701

[8]

DURST RA, 1990, FLOW INJECTION ANAL, V14, P181

[9]

EKINS RP, 1990, J CLIN IMMUNOASSAY, V13, P169

[10]

ENGLE SW, 1992, SUPERFUND 92

← 1 2 3 4 5 →