ASTM E2805-2011 Standard Practice for Measurement of the Biological Activity of Ricin《蓖麻蛋白生物活性的测量规程》.pdf
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1、Designation: E2805 11Standard Practice forMeasurement of the Biological Activity of Ricin1This standard is issued under the fixed designation E2805; the number immediately following the designation indicates the year oforiginal adoption or, in the case of revision, the year of last revision. A numbe
2、r in parentheses indicates the year of last reapproval. Asuperscript epsilon () indicates an editorial change since the last revision or reapproval.INTRODUCTIONRicin is a member of the protein toxins that cause their physiological effect by inactivation ofribosomes. Ricin is a member of the class 2
3、ribosome inactivating proteins (1).2Other members of thisclass of toxins include the proteins abrin and Shiga toxin.Ricin consists of two chains, the A-chain that is responsible for the N-glycosidase enzymaticactivity and the B-chain that is needed for cell binding and intra-cellular processing. Ric
4、in is aheterogeneous protein with molecular weights ranging from approximately 62 to 64 kilodaltons (kDa)(2). Both chains are glycosylated and of similar size (approximately 32 kDa). There are several genesencoding putative ricin and ricin-like proteins in the genome of R. communis (3) resulting ind
5、ifferences in the amino acid sequence of the subunits. The differences in amino acid sequence andglycosylation both contribute to the heterogeneity of ricin.1. Scope1.1 This guide is intended for the manufacturers and usersof ricin reference material. Ricin reference materials arewell-characterized
6、materials that can be used to test detectiondevices and calibrate laboratory measurements. It is anticipatedthat ricin reference materials will be characterized by bio-chemical methods in addition to the measurement of biologicalactivity.1.2 This practice details the measurement of ricin biologicala
7、ctivity using a cell-free translation (CFT) assay (4).1.3 The CFT assay has been developed for use in anybiotechnology laboratory where determination or confirmationof ricin biological activity is required.1.4 The CFT assay has been validated by the U.S. ArmyMedical Research Institute of Infectious
8、Diseases (USAM-RIID) VP-016 Validation of Cell-Free Translation Assay forthe Detection of Ricin Toxin Biological Activities in compli-ance (5) with Good Laboratory Practices (GLP) Regulations ofthe Food and Drug Administration (21 CFR Part 58). Strictadherence to the protocol is necessary for validi
9、ty of the testresults.1.5 Appendix X1 and Appendix X2 also provide guidancefor the measurement of the biological activity of ricin usingcell-based assays and the use of synthetic enzyme substrates.1.6 Ricin is a category 2 select agent and acquisition of thericin standard must adhere to the Center f
10、or Disease Control(CDC) regulations. Ricin is listed on the select agent list (42CFR Part 72).3The possession, transfer, and use of ricin arerestricted under the Public Health Security Preparedness Act(CRS Report RL31263 Public Health Security and Bioterror-ism Preparedness and Response Act (P.L. 10
11、7-188): Provisionand Changes to Preexisting law). Access to stores of ricin islimited (USA Patriot Act, P.L. 107-56). Ricin is also aprohibited substance under the Biological Weapons Conven-tion and the Chemical Weapons Convention (CRS ReportRL31559 Proliferation Control Regimes: Background andStatu
12、s).1.7 The values stated in SI units are to be regarded asstandard. No other units of measurement are included in thisstandard.1.8 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 a
13、ppro-priate safety and health practices and determine the applica-bility of regulatory limitations prior to use. Ricin is anextremely dangerous toxin. See Section 9 for specific hazardsinformation.2. Referenced Documents2.1 ASTM Standards:41This practice is under the jurisdiction of ASTM Committee E
14、54 on HomelandSecurity Applications and is the direct responsibility of Subcommittee E54.01 onCBRNE Sensors and Detectors.Current edition approved Jan. 1, 2011. Published March 2011. DOI: 10.1520/E2805-11.2The boldface numbers in parenthesis refer to the list of references at the end ofthis standard
15、.3Available at http:/www.bt.cdc.gov/Agent/agentlist.asp.4For referenced ASTM standards, visit the ASTM website, www.astm.org, orcontact ASTM Customer Service at serviceastm.org. For Annual Book of ASTMStandards volume information, refer to the standards Document Summary page onthe ASTM website.1Copy
16、right ASTM International, 100 Barr Harbor Drive, PO Box C700, West Conshohocken, PA 19428-2959, United States.F2149 Test Method for Automated Analyses of CellstheElectrical Sensing Zone Method of Enumerating and Siz-ing Single Cell Suspensions2.2 Code of Federal Regulations:21 CFR Part 58 Good labor
17、atory practice for nonclinicallaboratory studies542 CFR Part 72 Interstate shipment of etiologic agents62.3 ANSI/ATCC Standard:7ASN-0001-2009 Standardization of In-Vitro Assays to De-termine Anthrax Toxin Activities3. Terminology3.1 Abbreviations:3.1.1 CFTcell free translation.3.1.2 CPScounts per se
18、cond, units of luminescence in-strument.3.1.3 IC50concentration of ricin that produces inhibitionof 50 % of the activity in an assay.3.1.4 kDamolecular mass in kilo Dalton units.3.1.5 PBSphosphate buffered saline.4. Summary of Practice4.1 The CFT assay for measuring biologically active ricin isbased
19、 on its inhibitory effects on protein synthesis (6, 7). Whenadded to a rabbit reticulocyte translation mixture containingluciferase mRNA, ricin inhibits translation of the mRNA intothe enzyme luciferase. Luciferase is then detected using abuffer containing the luciferin substrate. The test is a biol
20、umi-nescence assay that measures the amount of luminescenceproportional to the amount of luciferase produced from proteintranslation (RNAprotein). When active ricin is present, theamount of luminescence decreases corresponding to a decreasein the production of the luciferase enzyme. The amount ofpro
21、tein (luciferase) produced is directly proportional to theamount of luminescence generated. The decrease in lumines-cence is directly proportional to the amount of active ricin inthe sample. Confirmation that translation inhibition is causedby the presence of active ricin is determined by mixing ana
22、liquot of the ricin samples with anti-ricin antibody beforeadding to the translation mixture. The neutralized ricin doesnot inhibit luciferase translation, and therefore, luminescencedoes not decrease.4.2 Cell-based assays use mammalian cells maintained inculture to measure the effect of ricin on ce
23、ll death or damage(cytotoxicity). Ricin is added to the cells and after an incuba-tion period, the effect on cell cytotoxicity is measured. Thericin-treated cells are compared to control cells (without addedricin) maintained under the same conditions. Guidance is givenin Appendix X1.4.3 The N-glycos
24、idase enzymatic activity of the A-chain ofricin can be measured using synthetic oligonucleotides. Theenzyme activity is measured either by the released adenine orthe effect on the depurinated substrate using a number ofmethods. Guidance is given in Appendix X2.5. Significance and Use5.1 The CFT assa
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