ASTM D6499-2003 Standard Test Method for the Immunological Measurement of Antigenic Protein in Natural Rubber and its Products《天然橡胶及其制品中抗原性蛋白质的免疫测量的标准试验方法》.pdf
《ASTM D6499-2003 Standard Test Method for the Immunological Measurement of Antigenic Protein in Natural Rubber and its Products《天然橡胶及其制品中抗原性蛋白质的免疫测量的标准试验方法》.pdf》由会员分享,可在线阅读,更多相关《ASTM D6499-2003 Standard Test Method for the Immunological Measurement of Antigenic Protein in Natural Rubber and its Products《天然橡胶及其制品中抗原性蛋白质的免疫测量的标准试验方法》.pdf(6页珍藏版)》请在麦多课文档分享上搜索。
1、Designation: D 6499 03Standard Test Method forThe Immunological Measurement of Antigenic Protein inNatural Rubber and its Products1This standard is issued under the fixed designation D 6499; the number immediately following the designation indicates the year oforiginal adoption or, in the case of re
2、vision, the year of last revision. A number in parentheses indicates the year of last reapproval. Asuperscript epsilon (e) indicates an editorial change since the last revision or reapproval.1. Scope1.1 This test method covers an immunological method todetermine the amount of antigenic protein in na
3、tural rubber andits products using rabbit antisera specific for natural rubberlatex (NRL) proteins. This immunoassay procedure quantita-tively measures the level of antigenic latex proteins in solutionusing an inhibition format. The samples may include glove orother rubber product extracts which hav
4、e been collected inorder to measure the latex protein levels. Although this methoddetects antigenic proteins, it should not be considered as ameasure of allergenic proteins. Correlation of protein/antigenlevels with the level of allergenic proteins has not been fullyestablished.1.2 For the purpose o
5、f this test method, the range of proteinwill be measured in terms of microgram to milligram quanti-ties.1.3 This standard does not purport to address all of thesafety concerns, if any, associated with its use. It is theresponsibility of the user of this standard to establish appro-priate safety and
6、health practices and determine the applica-bility of regulatory limitations prior to use.2. Referenced Documents2.1 ASTM Standards:D 4483 Practice For Determining Precision For TestMethod Standards in the Rubber and Carbon Black Indus-tries2D 5712 Test Method for Analysis of Aqueous ExtractableProte
7、in in Natural Rubber and its Products Using theModified Lowry Method33. Terminology3.1 Definitions:3.1.1 allergensprotein antigens which induce allergic im-mune reactions typically mediated through IgE antibodies.3.1.2 antibodyan immunoglobulin, a protein that is pro-duced as a part of the immune re
8、sponse which is capable ofspecifically combining with the antigen.3.1.3 antigenany substance that provokes an immuneresponse when introduced into the body.3.1.4 background absorbancethe absorbance reading inthe solution resulting from the presence of chemicals, ions etc.other than the substrate bein
9、g determined.3.1.5 blocking solutiona non-reactive protein solutionused to prevent nonspecific antibody adsorption.3.1.6 calibrationthe standardization of an instrument set-ting or an assay configuration.3.1.7 concentration rangethe recommended analyte con-centration range in g/mL that produces an a
10、bsorbance readingof 0.1 to 2.0 units.3.1.8 enzyme linked immunosorbent assay (ELISA)an im-munological test method to quantify antigen or antibody levelsusing an enzyme as the detection mechanism.3.1.9 primary antibodythe antibody used first in a se-quence that is specific for the antigen.3.1.10 refe
11、rence solutionthe solution to which the testsample is being compared against.3.1.11 repeatabilitythe variability or test error betweenindependent test results obtained within a single laboratory.3.1.12 reproducibilitythe variability or error between testresults obtained in different laboratories.3.1
12、.13 secondary antibodythe enzyme conjugated anti-body used second in the sequence that is specific for the heavychain of the primary antibody.3.1.14 standard solutionthe preparation of standard ana-lyte used as a reference to which the unknown sample beingmeasured is compared.3.1.15 substratethe mat
13、erial or substance upon which anenzyme reacts.3.1.16 titerthe strength of the antibody solution (forexample, concentration and affinity of antibody).1This specification is under the jurisdiction of ASTM Committee D11 on Rubber, and is the direct responsibility of Subcommittee D11.40 on Consumer Rubb
14、erProducts.Current edition approved June 10, 2003. Published June 2003. Originallyapproved in 2000. Last previous edition approved in 2000 as D 6499 00.2Annual Book of ASTM Standards, Vol 09.01.3Annual Book of ASTM Standards, Vol 09.02.1Copyright ASTM International, 100 Barr Harbor Drive, PO Box C70
15、0, West Conshohocken, PA 19428-2959, United States.4. Summary of Test Method4.1 The latex device is extracted for2hinanaqueousbuffer. The extract is recovered and the antigen levels aredetermined using inhibition Enzyme Linked ImmunoSorbentAssay (ELISA) technology (1).4The ELISA assay is based onpol
16、yclonal antiserum which can detect NRL proteins. ELISAtechnology takes advantage of the specificity and sensitivity ofthe antibody-antigen reaction. A variation of the ELISAmethod (an inhibition ELISA) has been developed for thedetection and quantification of latex protein antigens. In theinhibition
17、 ELISA, the latex antigen is immobilized by absorp-tion to the wells of a 96-well test plate. The sample extract ismixed with antibody specific for NRL protein in a dilutionplate. Following a brief incubation to allow for antibodyrecognition of the relevant NRL antigens, the mixture is addedto the i
18、mmobilized antigen in the assay plate. Anti-NRLantibody which is not bound to the soluble NRL protein in thesample will bind to the immobilized antigen. The plate iswashed to remove the soluble antigen antibody complexes anda secondary antibody (enzyme-labeled anti-immunoglobulin)is added which atta
19、ches to the immobilized antigen-boundspecific antibody. Next, the enzyme substrate is added and thereaction of the enzyme on the substrate results in a colorchange. A reduction in the amount of color in comparison to anuninhibited control is an indicator of the amount of antigenpresent in the sample
20、. Comparison to a standard curve gener-ated using known amounts of NRL protein permits quantifica-tion. The assay is highly sensitive and can quantitate NRLproteins in the nanogram per millilitre range.5. Significance and Use5.1 Type 1 latex allergy most commonly manifests aslocalized urticaria afte
21、r contact of skin with natural rubber butcan also include symptoms of allergic rhinoconjunctivitis,asthma and rarely anaphylaxis. This immediate (Type I) allergyis caused by natural proteins inherent to the rubber tree, whichremain on the finished natural rubber products. The quantifi-cation of prot
22、ein levels in NRL products using the standardcolorimetric protein assays may give spurious results due tochemical additives in the latex formulations that interfere withthe assay (2,3). Furthermore, the amount of protein found inNRL products are often below the detection limits of thestandard colori
23、metric protein assay (4,5).5.2 This test method describes an immunological methodfor quantitation of natural rubber latex proteins using rabbitanti-NRL serum. Rabbits immunized with NRL proteins reactto the majority of the proteins present, and their sera have thecapability to detect most if not all
24、 of the proteins in NRL.Therefore, although rabbit antibody reacts with antigenicmaterial, this should not be considered as quantitative measureof total protein levels.6. Interferences6.1 Substances such as detergents or surfactants have thepotential to prevent antibody binding to antigen and couldi
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