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ASTM F2131-02(2007)

(Test Method)

Standard Test Method forIn Vitro Biological Activity of Recombinant Human Bone Morphogenetic Protein-2 (rhBMP-2) Using the W-20 Mouse Stromal Cell Line

Standard Test Method for<bdit>In Vitro</bdit> Biological Activity of Recombinant Human Bone Morphogenetic Protein-2 (rhBMP-2) Using the W-20 Mouse Stromal Cell Line

SCOPE
1.1 This test method describes the method used and the calculation of results for the determination of the  in vitro biological activity of rhBMP-2 using the mouse stromal cell line W-20 clone 17 (W-20-17). This clone was derived from bone marrow stromal cells of the W++ mouse strain.
1.2 This test method (assay) has been qualified and validated based upon the International Committee on Harmonization assay validation guidelines (with the exception of interlaboratory precision) for the assessment of the biological activity of rhBMP-2. The relevance of this in vitro test method to in vivo bone formation has also been studied. The measured response in the W-20 bioassay, alkaline phosphatase induction, has been correlated with the ectopic bone-forming capacity of rhBMP-2 in the in vivo Use Test (UT). rhBMP-2 that was partially or fully inactivated by targeted peracetic acid oxidation of the two methionines was used as a tool to compare the activities. Oxidation of rhBMP-2 with peracetic acid was shown to be specifically targeted to the methionines by peptide mapping and mass spectrometry. These methionines reside in a hydrophobic receptor binding pocket on rhBMP-2. Oxidized samples were compared alongside an incubation control and a native control. The 62, 87, 98, and 100 % oxidized samples had W-20 activity levels of 62, 20, 7, and 5 %, respectively. The incubation and native control samples maintained 100 % activity. Samples were evaluated in the UT and showed a similar effect of inactivation on bone-forming activity. The samples with 62 % and 20 % activity in the W-20 assay demonstrated reduced levels of bone formation, similar in level with the reduction in W-20 specific activity, relative to the incubation control. Little or no ectopic bone was formed in the 7 and 5 % active rhBMP-2 implants.
1.3 Thus, modifications to the rhBMP-2 molecule in the receptor binding site decrease the activity in both the W-20 and UT assays. These data suggest that a single receptor binding domain on rhBMP-2 is responsible for both in vitro and in vivo activity and that the W-20 bioassay is a relevant predictor of the bone-forming activity of rhBMP-2.
1.4 The values stated in SI units are to be regarded as standard.
This standard does not purport to address all of the safety concerns, if any, associated with its use. It is the responsibility of the user of this standard to establish appropriate safety and health practices and determine the applicability of regulatory limitations prior to use.

General Information

Status
Historical
Publication Date
31-Jan-2007
ICS
07.080 - Biology. Botany. Zoology
Technical Committee
F04 - Medical and Surgical Materials and Devices
Drafting Committee
F04.42 - Biomaterials and Biomolecules for TEMPs
Current Stage
Ref Project

Relations

Replaces
ASTM F2131-02 - Standard Test Method for<bdit>In Vitro</bdit> Biological Activity of Recombinant Human Bone Morphogenetic Protein-2 (rhBMP-2) Using the W-20 Mouse Stromal Cell Line
Effective Date
01-Feb-2007
Replaced By
ASTM F2131-02(2007)e1 - Standard Test Method for<bdit>In Vitro</bdit> Biological Activity of Recombinant Human Bone Morphogenetic Protein-2 (rhBMP-2) Using the W-20 Mouse Stromal Cell Line
Effective Date
01-Feb-2007
Referred By
ASTM F2529-13(2021) - Standard Guide for  <emph type="ital"> in vivo</emph> Evaluation of Osteoinductive Potential for Materials Containing Demineralized Bone (DBM)
Effective Date
01-Feb-2007
Referred By
ASTM F2211-13(2021) - Standard Classification for Tissue-Engineered Medical Products (TEMPs)
Effective Date
01-Feb-2007

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ASTM F2131-02(2007) - Standard Test Method for<bdit>In Vitro</bdit> Biological Activity of Recombinant Human Bone Morphogenetic Protein-2 (rhBMP-2) Using the W-20 Mouse Stromal Cell LineASTM F2131-02(2007) - Standard Test Method for<bdit>In Vitro</bdit> Biological Activity of Recombinant Human Bone Morphogenetic Protein-2 (rhBMP-2) Using the W-20 Mouse Stromal Cell Line
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ASTM F2131-02(2007) - Standard Test Method for<bdit>In Vitro</bdit> Biological Activity of Recombinant Human Bone Morphogenetic Protein-2 (rhBMP-2) Using the W-20 Mouse Stromal Cell Line
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NOTICE: This standard has either been superseded and replaced by a new version or withdrawn.
Contact ASTM International (www.astm.org) for the latest information
Designation:F2131–02 (Reapproved 2007)
Standard Test Method for
In Vitro Biological Activity of Recombinant Human Bone
Morphogenetic Protein-2 (rhBMP-2) Using the W-20 Mouse
Stromal Cell Line
This standard is issued under the fixed designation F2131; the number immediately following the designation indicates the year of
original adoption or, in the case of revision, the year of last revision.Anumber in parentheses indicates the year of last reapproval.A
superscript epsilon (e) indicates an editorial change since the last revision or reapproval.
1. Scope control. Little or no ectopic bone was formed in the 7 and 5%
active rhBMP-2 implants.
1.1 This test method describes the method used and the
1.3 Thus, modifications to the rhBMP-2 molecule in the
calculation of results for the determination of the in vitro
receptorbindingsitedecreasetheactivityinboththeW-20and
biological activity of rhBMP-2 using the mouse stromal cell
UT assays. These data suggest that a single receptor binding
line W-20 clone 17 (W-20-17). This clone was derived from
2 domainonrhBMP-2isresponsibleforbothinvitroandinvivo
bone marrow stromal cells of the W++ mouse strain.
activity and that the W-20 bioassay is a relevant predictor of
1.2 This test method (assay) has been qualified and vali-
the bone-forming activity of rhBMP-2.
dated based upon the International Committee on Harmoniza-
1.4 The values stated in SI units are to be regarded as
tion assay validation guidelines (with the exception of inter-
standard.
laboratory precision) for the assessment of the biological
1.5 This standard does not purport to address all of the
activity of rhBMP-2.The relevance of this in vitro test method
safety concerns, if any, associated with its use. It is the
to in vivo bone formation has also been studied. The measured
responsibility of the user of this standard to establish appro-
responseintheW-20bioassay,alkalinephosphataseinduction,
priate safety and health practices and determine the applica-
has been correlated with the ectopic bone-forming capacity of
bility of regulatory limitations prior to use.
rhBMP-2 in the in vivo Use Test (UT). rhBMP-2 that was
partially or fully inactivated by targeted peracetic acid oxida-
2. Terminology
tion of the two methionines was used as a tool to compare the
2.1 rhBMP—recombinant human bone morphogenetic pro-
activities. Oxidation of rhBMP-2 with peracetic acid was
tein.
showntobespecificallytargetedtothemethioninesbypeptide
2.2 GDF—growth and differentiation factor.
mappingandmassspectrometry.Thesemethioninesresideina
hydrophobic receptor binding pocket on rhBMP-2. Oxidized
3. Summary of Test Method
samples were compared alongside an incubation control and a
3.1 Inthistestmethod,themousestromalcelllineW-20-17
nativecontrol.The62,87,98,and100%oxidizedsampleshad
is used as a target cell line for rhBMP-2. The W-20-17 cells
W-20 activity levels of 62, 20, 7, and 5%, respectively. The
exhibit increased alkaline phosphatase activity in response to
incubation and native control samples maintained 100% ac-
rhBMP-2. Optical density at 405 nm of the p-nitrophenol
tivity. Samples were evaluated in the UTand showed a similar
generated from the alkaline phosphatase substrate is used as a
effect of inactivation on bone-forming activity. The samples
measure of alkaline phosphatase enzyme level. The test
with 62% and 20% activity in the W-20 assay demonstrated
method is performed in a 96-well plate format. A similar test
reduced levels of bone formation, similar in level with the
methodbaseduponthesamecelllinehasbeendevelopedusing
reduction in W-20 specific activity, relative to the incubation
chemiluminescent detection of alkaline phosphatase.
4. Significance and Use
ThistestmethodisunderthejurisdictionofASTMCommitteeF04onMedical
4.1 Although the test method can be used for assessment of
andSurgicalMaterialsandDevicesandisthedirectresponsibilityofSubcommittee
the bioactivity of crude preparations of rhBMP-2, it has only
F04.42 on Biomaterials and Biomolecules for TEMPs.
been validated for use with highly pure (>98% by weight
Current edition approved Feb. 1, 2007. Published February 2007. Originally
approved in 2002. Last previous edition approved in 2002 as F2131–02.
protein purity) preparations of rhBMP-2.
Thies, R. S., Bauduy, M., Ashton, B. A., Kurtzberg, L., Wozney, J.M., and
Rosen, V., “Recombinant Human Bone Morphogenetic Protein-2 Induces Osteo-
blastic Differentiation in W-20-17 Stromal Cells,” Endocrinology, 130, 1992, pp.
1318-1324. Blum, R. S., Li, R. H., Mikos,A.G., and Barry, M.A., “An Optimized Method
Guideline for Industry, ICH-Q2AText on Validation ofAnalytical Procedures, for the Chemiluminescent Detection of Alkaline Phosphatase Levels During
November 1996, International Committee on Harmonization, March 1995, http:// Osteodifferentiation by Bone Morphogenetic Protein 2,” Jour. Cellular Biochem.,
www.fda.gov/cder/guidance/index/htm. 80, 2001, pp. 532-537.
Copyright © ASTM International, 100 Barr Harbor Drive, PO Box C700, West Conshohocken, PA 19428-2959, United States.
F2131–02 (2007)
5. Interferences 7.6 200 mM L-Glutamine (Invitrogen Life Technologies,
25030081 or equivalent).
5.1 There have been no systematic studies of interfering
7.7 Gentamicin Gibco sterile filtered: 10 mg/mL or equiva-
substances for this test method. There is anecdotal evidence
lent.
that trypsin and some rhBMP-2 formulation buffers can inter-
7.8 Penicillin Streptomycin (PS), contains 10 000 units of
fere with the assay. Additionally, the source of fetal bovine
penicillin(base)/mLand10000µgofstreptomycin(base)/mL,
serum is an important variable. Each lot should be tested in all
utilizing penicillin G (sodium salt) and streptomycin sulfate in
parts of the assay where it is required to determine the
0.85 % saline (Invitrogen Life Technologies, #15140122 or
appropriateness of the lot. This is particularly needed if fetal
equivalent).
bovine serum vendor is changed.
7.9 Phosphate Buffered Saline, Calcium and Magnesium
Free, 1x (PBS-CMF), (Invitrogen Life Technologies (cat.
6. Apparatus
#20012050 or equivalent).
6.1 Polypropylene conical tubes, 15 mL and 50 mL.
7.10 Dimethyl sulfoxide (DMSO), cell culture grade
6.2 Cryovials (Corning or equivalent), sterile 2 mL.
(Sigma-Aldrich or equivalent).
6.3 Eppendorf vials, sterilized.
7.11 Trypsin-EDTA(0.05%trypsin,0.53mMEDTA·4Na)
6.4 Variablepipets,(range20to1000µL)andMultichannel
(1X), liquid (Invitrogen Life Technologies 25300054 or
pipets (range 50 to 300 µL).
equivalent).
6.5 Biosafety cabinet.
7.12 Glycine (Sigma —Aldrich or equivalent).
6.6 96 Well flat bottom sterile tissue culture microtiter
7.13 Sodium Hydroxide (NaOH) 0.2 N and 10 N.
plates, (Falcon 3072 or equivalent).
7.14 Triton X-100 (J.T. Baker Cat. No. X198-05 or equiva-
6.7 IEC Centra-7R Centrifuge, or equivalent.
lent).
6.8 CO humidified tissue culture incubator.
7.15 Magnesium Chloride, Crystalline (MgCl·6H O).
2 2
6.9 Spectrophotometric microplate reader, (VMAX/
7.16 p-Nitrophenol phosphate (PNPP, Sigma—Aldrich
Spectramax, Molecular Devices, or equivalent).
104(R) phosphatase substrate, product # 1040 or equivalent).
6.10 Hemacytometer, or automatic cell counter.
7.17 NaCl.
6.11 Inverted microscope.
7.18 Purified water.
6.12 Tissue culture flasks, Falcon T175 or equivalent.
7.19 rhBMP-2, 1st WHO Reference Reagent 1997 (5000
6.13 Sterilized paper towels, or equivalent.
Units per ampoule, cat. # 93/574, National Institute for
6.14 Sterile filter units, (0.2 µm).
Biological Standards and Control).
6.15 Sterile pipets, (1 mL, 5 mL, 10 mL, 25 mL, 50 mL).
7.20 rhBMP-2 internal control, >1 mg/mL (stored at
6.16 9 in. Pasteur pipets, sterilized.
−80°C).
6.17 Sterilized pipet tips, (1-300 µL and 200-1000 µL).
6.18 Sterile reagent reservoirs.
8. Procedure
6.19 −80°C freezer.
6.20 96 Well U-Bottom polypropylene sterile tissue culture
8.1 Solution Preparation:
microtiter plates, (Costar 3790 or equivalent).
8.1.1 DME Low Bicarb:
6.21 Water bath.
8.1.1.1 Dissolve 66.87 g DME/High and 11.13 g sodium
6.22 Orbital shaker.
bicarbonate in 4.5 L of purified water.
8.1.1.2 Adjust pH to 7.3 6 0.10 with 5 M HCl and bring
7. Reagents and Materials
solution to 5 L with purified water.
7.1 W-20-17 Mouse Stromal Cells.
8.1.1.3 Filter through a 0.2 µm filter into sterile bottles.
7.2 Dulbecco’s modified Eagle’s medium with 4500 mg/L
8.1.1.4 Store at 2 to 8°C, expires in 8 weeks.
glucose and 4.0 mM L-glutamine, without sodium bicarbonate
8.1.2 Hi FBS:
(DME/High, JRH Biosciences, 56439 or equivalent).
8.1.2.1 Thaw the desired amount of FBS at ambient tem-
7.3 Sodium bicarbonate (Sigma—Aldrich S4019 or equiva-
perature, or 2 to 8°C.
lent).
8.1.2.2 Adjust the waterbath to a temperature of 56 6 2°C.
7.4 5 M hydrochloric acid.
8.1.2.3 PlacethebottleofFBSintothewaterbathsothatthe
7.5 Heat inactivated (Hi) fetal bovine serum (FBS).
entire contents of the bottle are immersed in water.
8.1.2.4 Heat the bottle for 45 min, swirling periodically.
NOTE 1—Each new lot of fetal bovine serum must be evaluated in the
assay before use.
Thismaterialhasbeenfoundsatisfactoryforthispurposeandisavailablefrom
This cell line has been deposited in mid-2001 at the American Type Culture Invitrogen Life Technologies, 1600 Faraday Ave., P.O. Box 6482, Carlsbad, CA
Collection, 10801 University Blvd., Manassas, VA 20110-2209, U.S., http:// 92008, U.S., http://www.invitrogen.com.
www.atcc.org. Thismaterialhasbeenfoundsatisfactoryforthispurposeandisavailablefrom
Thismediumhasbeenfoundsatisfactoryforthispurposeandisavailablefrom J.T.Baker,(MallinckrodtBaker,Inc.),222RedSchoolLn.,Phillipsburg,NJ08865,
JRHBiosciences,P.O.Box14848,Lenexa,KS66215,U.S.,http://www.jrhbio.com. U.S., http://www.jtbaker.com.
7 10
Thismaterialhasbeenfoundsatisfactoryforthispurposeandisavailablefrom Thismaterialhasbeenfoundsatisfactoryforthispurposeandisavailablefrom
Sigma-Aldrich Corp., 3050 Spruce St., St. Louis, MO 63103, U.S., http:// the National Institute for Biological Standards and Control (NIBSC), Blanche Ln.,
www.sigmaaldrich.com. South Mimms, Potters Bar, Herts, EN6 3QG, U.K., http://www.nibsc.ac.uk.
F2131–02 (2007)
8.1.2.5 Remove the bottle from the waterbath, allow to cool 8.1.9.2 Add 0.34% (w/v) p-nitrophenol phosphate within
to room temperature. Aliquot 50 mL of the FBS in sterile 50 one (1) h of use and mix well.
mL conical tubes.
NOTE 2—Assay mix must be made on day of use.
8.1.2.6 Label each container with name, lot number, expi-
Component Example: 50 mL for 10 plates
rationdate,andtheheatinactivationdate.Storeat−20 610°C
Glycine buffer 50 mL
PNPP substrate 170 mg
or 2 to 8°C.
8.1.3 Growth Medium:
8.2 Cell Line Storage and Cell Banking Procedure:
8.1.3.1 Combine the following components in the corre-
8.2.1 Store the cells in 1 mLaliquots in 2 mLcryovials at 5
sponding proportions (v/v):
3 10 cells/mL in freezing medium (see 8.1.7).
Component Proportion (% v/v) Example: 500 mL (mL) 8.2.2 Prepare cells to make a working cell bank (100+
DME Low Bicarb 85.5 427.5
vials).
Hi FBS 10.0 50.0
8.2.3 Thaw the vial of W-20-17 cells obtained from ATCC
L-Glutamine (200 mM) 4.0 20.0
Gentamicin 0.5 2.5 or other source following the procedure described in 8.3.
8.2.4 Inordertoobtaintheexpectedcellnumber,subculture
8.1.3.2 Filter through a 0.2 µm filter and store at 2 to 8°C in
the cells by expanding them through one or two additional
a sterile container.
passages (repeat steps in 8.3).
8.1.4 Assay Medium:
8.1.4.1 Combine the following components in the corre- NOTE 3—The viability should be in the range$80%.
sponding proportions (v/v):
8.2.5 Determine the number of vials to be made based on
Component Proportion (% v/v) Example: 1000 mL (mL)
totalcellnumberobtainedfollowingprocedure8.2.2.Labelthe
DME Low Bicarb 87.0 870.0
appropriate number of cryovials as follows:
Hi FBS 10.0 100.0
L-Glutamine (200 mM) 2.0 20.0
Cell Line Name WCB
Penicillin/streptomycin 1.0 10.0
Passage Number
Freezing Date
8.1.4.2 Filter through a 0.2 µm filter and store at 2 to 8°C in
Preparation Reference Number
a sterile container. Initials
8.1.5 NaCl, 0.9% w/v:
8.2.6 Decap the cryovials in the biosafety cabinet.
8.1.5.1 Dissolve 9 g NaCl in approximately 800 mL of
8.2.7 Dilute the cell suspension to one half the appropriate
purified water and bring to a final volume of 1 Lwith purified
volume with 2 to 8°C cold freezing medium without DMSO.
water.
Volume should be one half of the appropriate volume for the
8.1.5.2 Filter through a 0.2 µm filter and store in a sterile
desired cell suspension for freezing. The second half of the
container at room temperature.
cold freezing medium should be made with culture medium
8.1.6 12.5% Triton X-100:
(see 8.1.7, 20% DMSO, the final DMSO concentration must
8.1.6.1 Mix 12.5 mL Triton X-100 with 87.5 mL of 0.9%
be 10%).
NaCl.
8.2.8 Slowly add the half-volume of culture medium with
8.1.6.2 Filter through a 0.2 µm filter and store in a sterilized
20% DMSO to the other half of the volume of the cell
container at room temperature.
suspension.
8.1.7 Freezing Medium:
8.2.9 Using a sterile pipet, transfer 1 mL of cell suspension
8.1.7.1 Prepare freezing medium immediately before freez-
toeachofthelabeledcryovialsonice.Repeatuntilallvialsare
ing procedure by adding DMSO to growth medium (see 9.1.3)
filled. Gently mix the cell suspension during the filling process
to 20% v/v.
to prevent settling of the cells.
Component Proportion (% v/v) Example: 100 mL
NOTE 4—TheperiodoftimefromtheadditionoftheDMSOcontaining
Growth Medium 80 80 mL
medium to the start of freezing process should not exceed 45 to 60 min.
DMSO 20 20 mL
8.2.10 Transfer the cryovials to an insulated box or rack.
8.1.8 Glycine Buffer:
Store the box or rack at −80°C for 20 to 24 h.
8.1.8.1 Dissolve0.75%(w/v)glycineinrequiredvolumeof
8.2.11 After20to24h,transferthevialstoaliquidnitrogen
purifiedwater.AdjustthepHofthesolutionto10.3 60.1with
dewar or freezer.
10 N NaOH.
8.2.12 Perform test thaws to check the viability and assay
8.1.8.2 Add 0.8% (v/v) of 12.5% Triton X-100.
performance of cells.
8.1.8.3 Add 0.13% (w/v) MgCl·6H O and mix well.
2 2
Component Example: 1000 mL
NOTE 5—It is recommended to perform mycoplasma and sterility
Glycine 7.5 g
testing on the new bank.
MgCl·6H O 1.3 g
2 2
12.5 % Triton X-100 8.0 mL
8.3 Preparation of Cells for the Assay:
Water To 1000 mL
8.3.1 Two vials of cells (W-20-17, stored in liquid nitrogen)
8.1.8.4 Filter through a 0.2 µm filter and store in a sterile are quick thawed in a 37 6 2°C waterbath.The contents of the
container at room temperature. One month expiration.
vials are combined in a 15 mL conical tube and mixed
8.1.9 Assay Mix: thoroughly. The total volume is recorded.
8.1.9.1 Take a sufficient volume of the glycine buf
...

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Standard Test Method for In Vitro Biological Activity of Recombinant Human Bone Morphogenetic Protein-2 (rhBMP-2) Using the W-20 Mouse Stromal Cell Line

SIGNIFICANCE AND USE
4.1 Although the test method can be used for assessment of the bioactivity of crude preparations of rhBMP-2, it has only been validated for use with highly pure (>98 % by weight protein purity) preparations of rhBMP-2.
SCOPE
1.1 This test method describes the method used and the calculation of results for the determination of the in-vitro biological activity of rhBMP-2 using the mouse stromal cell line W-20 clone 17 (W-20-17). This clone was derived from bone marrow stromal cells of the W++ mouse strain.2  
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Standard Guide for Assessing the Attachment of Cells to Biomaterial Surfaces by Physical Methods

SIGNIFICANCE AND USE
4.1 Cell attachment or, lack of it, to biomaterials is a critical factor affecting the performance of a device or implant. Cell attachment is a complicated, time-dependent, process involving significant morphological changes of the cell and deposition of a bed of extracellular matrix. Details of the adhesive bond that is formed have been reviewed by, for example, Pierres et al (2002) (4), Lukas and Dvorak (2004) (5), and Garcia and Gallant (2003) (6). The strength of this coupling can be determined either by monitoring the force of attachment between a cell and a substrate over time or by measuring the force required to detach the cell once it has adhered.  
4.2 Cell adhesion to a surface depends on a range of biological and physical factors that include the culture history, the age of the cell, the cell type, and both the chemistry and morphology of the underlying surface and time. These elements need to be considered in developing a test protocol.  
4.3 Devising robust methods for measuring the propensity of cells to attach to different substrates is further complicated since either cell adhesion or detachment can be assessed. These processes are not always similar or complementary.  
4.4 Most studies of cell attachment focus on obtaining some measure of the time-dependent force required to detach, or de-adhere, cells that have already adhered to a surface (James et al, 2005) (7). More recently investigators have begun to measure the adhesive forces that develop between cells and the underlying surface during attachment (Lukas and Dvorak, 2004) (5). From a practical point of view, it is much easier to measure the force required to detach or de-adhere cells from a surface than to measure those that develop during attachment. However, in both cases, the experimental data should be interpreted with a degree of caution that depends on the intended use of the measurements. The methods of measuring cell adhesion described herein are measures of the force required to ...
SCOPE
1.1 This guide describes protocols that can be used to measure the strength of the adhesive bond that develops between a cell and a surface as well as the force required to detach cells that have adhered to a substrate. Controlling the interactions of mammalian cells with surfaces is fundamental to the development of safe and effective medical products. This guide does not cover methods for characterizing surfaces. The information generated by these methods can be used to obtain quantitative measures of the susceptibility of surfaces to cell attachment as well as measures of the adhesion of cells to a surface. This guide also highlights the importance of cell culture history and influences of cell type.  
1.2 This standard does not purport to address all of the safety concerns, if any, associated with its use. It is the responsibility of the user of this standard to establish appropriate safety, health, and environmental practices and determine the applicability of regulatory limitations prior to use.  
1.3 This international standard was developed in accordance with internationally recognized principles on standardization established in the Decision on Principles for the Development of International Standards, Guides and Recommendations issued by the World Trade Organization Technical Barriers to Trade (TBT) Committee.

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ASTM
ASTM E1262-88(2018)(Guide)
Standard Guide for Performance of Chinese Hamster Ovary Cell/Hypoxanthine Guanine Phosphoribosyl Transferase Gene Mutation Assay

SIGNIFICANCE AND USE
2.1 The CHO/HGPRT assay detects forward mutations of the X-linked hypoxanthine-guanine phosphoribosyl transferase (hgprt) locus (coding for the enzyme, HGPRT) in Chinese hamster ovary (CHO) cells. Cells originally derived from Chinese hamster ovary tissue are exposed to a test article and, following an appropriate cell culture regimen, descendants of the original treated population are monitored for the loss of functional HGPRT, presumably due to mutations. Resistance to a purine analogue, 6-thioguanine (6TG) (or less desirably, 8-azaguanine (8AG)), is employed as the genetic marker. HGPRT catalyzes the conversion of the nontoxic 6TG to its toxic ribophosphorylated derivative. Loss of the enzyme or its activity therefore leads to cells resistant to 6TG.  
2.2 Because HGPRT is an enzyme of the purine nucleotide salvage pathway, loss of the enzyme is not a lethal event. Different types of mutational events (base substitutions, frameshifts, deletions, some chromosomal type lesions, and so forth) should theoretically be detectable at the hgprt locus. The CHO/HGPRT assay has been used to study a wide range of mutagens, including radiations (2-4), and a wide variety of chemicals (1), and complex chemical mixtures (5).
SCOPE
1.1 This guide highlights some of the more relevant biological concepts as they are currently understood, and summarizes the critical technical aspects for acceptable bioassay performances as they currently are perceived and practiced. The Chinese hamster ovary cell/hypoxanthine guanine phosphoribosyl transferase (CHO/HGPRT) assay (1) 2 has been widely applied to the toxicological evaluation of industrial and environmental chemicals.  
1.2 This guide concentrates on the practical aspects of cell culture, mutagenesis procedures, data analysis, quality control, and testing strategy. The suggested approach represents a consensus of the panel members for the performance of the assay. It is to be understood, however, that these are merely general guidelines and are not to be followed without the use of sound scientific judgement. Users of the assay should evaluate their approach based on the properties of the substances to be tested and the questions to be answered.  
1.3 Deviation from the guidelines based on sound scientific judgement should by no means invalidate the results obtained.  
1.4 The values stated in SI units are to be regarded as standard. No other units of measurement are included in this standard.  
1.5 This standard does not purport to address all of the safety concerns, if any, associated with its use. It is the responsibility of the user of this standard to establish appropriate safety, health, and environmental practices and determine the applicability of regulatory limitations prior to use.  
1.6 This international standard was developed in accordance with internationally recognized principles on standardization established in the Decision on Principles for the Development of International Standards, Guides and Recommendations issued by the World Trade Organization Technical Barriers to Trade (TBT) Committee.

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ASTM F748-16(Practice)
Standard Practice for Selecting Generic Biological Test Methods for Materials and Devices

SIGNIFICANCE AND USE
4.1 The objective of this practice is to recommend appropriate biological endpoint assessments (which may or may not require testing) to establish a reasonable level of confidence concerning the biological response to a material or device, while at the same time avoiding unnecessary testing.  
4.2 This practice is intended to provide guidance to the materials investigator in selecting the proper procedures to be carried out for the screening of new or modified materials. Because each material and each implant situation involves its own unique circumstances, these recommendations should be modified as necessary and do not constitute the only assessment that will be required for a material. Nor should these guidelines be interpreted as minimum requirements for any particular situation. While an attempt has been made to provide recommendation for different implant circumstances, some of the recommended assessment may not be necessary or reasonable for a specific material or application.
SCOPE
1.1 This practice recommends generic biological test methods for materials and devices according to end-use applications. While chemical testing for extractable additives and residual monomers or residues from processing aids is necessary for most implant materials, such testing is not included as part of this practice. The reader is cautioned that the area of materials biocompatibility testing is a rapidly evolving field, and improved methods are evolving rapidly, so this practice is by necessity only a guideline. A thorough knowledge of current techniques and research is critical to a complete evaluation of new materials.  
1.2 These test protocols are intended to apply to materials and medical devices for human application. Biological evaluation of materials and devices, and related subjects such as pyrogen testing, batch testing of production lots, and so on, are also discussed. Tests include those performed on materials, end products, and extracts. Rationale and comments on current state of the art are included for all test procedures described.  
1.3 The biocompatibility of materials used in single or multicomponent medical devices for human use depends to a large degree on the particular nature of the end-use application. Biological reactions that are detrimental to the success of a material in one device application may have little or no bearing on the successful use of the material for a different application. It is, therefore, not possible to specify a set of biocompatibility test methods which will be necessary and sufficient to establish biocompatibility for all materials and applications.  
1.4 The evaluation of tissue engineered medical products (TEMPs) may, in some cases, involve different or additional testing beyond those suggested for non-tissue-based materials and devices. Where appropriate, these differences are discussed in this practice and additional tests described.  
1.5 The ethical use of research animals places the obligation on the individual investigator to determine the most efficient methods for performing the necessary testing without undue use of animals. Where adequate prior data exists to substantiate certain types of safety information, these guidelines should not be interpreted to mean that testing should be unnecessarily repeated.  
1.6 This standard does not purport to address all of the safety concerns, if any, associated with its use. It is the responsibility of the user of this standard to establish appropriate safety and health practices and determine the applicability of regulatory limitations prior to use.

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ASTM
ASTM E1705-23(Terminology)
Standard Terminology Relating to Bioenergy and Industrial Chemicals from Biomass

SCOPE
1.1 This document is composed of terms, definitions of terms, descriptions of terms, and acronyms used in ASTM documents related to the field of bioenergy and industrial chemicals from biomass. Terms that are adequately defined in a general dictionary are not defined in this terminology standard.  
1.2 This standard includes terminology used in areas related to bioenergy and industrial chemicals from biomass, such as, but not limited to: characterization and identification of biomass, aseptic sampling, preservation of biological samples, sustainability, denatured fuel ethanol, cooking fuels and biomass conversion.  
1.2.1 The bylaws for Committee E48 allow the definitions approved in current E48 standards to be added to this terminology standard editorially. The definitions will have an attribution to indicate the standard(s) containing the definition. Subcommittee E48.91 can also develop definitions for the terminology standard. Those definitions will be attributed to the subcommittee.  
1.3 This international standard was developed in accordance with internationally recognized principles on standardization established in the Decision on Principles for the Development of International Standards, Guides and Recommendations issued by the World Trade Organization Technical Barriers to Trade (TBT) Committee.

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ASTM
ASTM E943-23(Terminology)
Standard Terminology Relating to Biological Effects and Environmental Fate

SCOPE
1.1 This terminology document defines terms commonly used in standards developed by ASTM Subcommittee E50.47 on Biological Effects and Environmental Fate. This terminology document is intended to be consistent with the use of terms in ASTM standards related to this field and, to the extent possible, with use by other organizations.  
1.1.1 If a specific Subcommittee E50.47 standard uses one of these terms in a different context, then the term should be defined in that standard. A term used only in a specific ASTM standard need not be included in this terminology document.  
1.2 This international standard was developed in accordance with internationally recognized principles on standardization established in the Decision on Principles for the Development of International Standards, Guides and Recommendations issued by the World Trade Organization Technical Barriers to Trade (TBT) Committee.

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ASTM E729-23e1(Guide)
Standard Guide for Conducting Acute Toxicity Tests on Test Materials with Fishes, Macroinvertebrates, and Amphibians

SIGNIFICANCE AND USE
5.1 An acute toxicity test is conducted to obtain information concerning the immediate effects on test organisms of a short-term exposure to a test material under specific experimental conditions. An acute toxicity test does not provide information about whether delayed effects will occur, although a post-exposure observation period, with appropriate feeding, if necessary, might provide such information. Bioavailability of the test substance may also differ between real-world exposures and laboratory exposures due to site-specific water quality conditions (see Guides E1192, E1563, and E2455).  
5.2 Results of acute toxicity tests might be used to predict acute effects likely to occur on aquatic organisms in field situations as a result of exposure under comparable conditions, except that (1) motile organisms might avoid exposure when possible, and (2) toxicity to benthic organisms might be dependent on sorption or settling of the test material onto the substrate.  
5.3 Results of acute tests might be used to compare the acute sensitivities of different species and the acute toxicities of different test materials, and to study the effects of various environmental factors on results of such tests.  
5.4 Results of acute toxicity tests might be an important consideration when assessing the hazards of materials to aquatic organisms (see Guide E1023) or when deriving water quality criteria for aquatic organisms (3).  
5.5 Results of acute toxicity tests might be useful for studying the biological availability of, and structure-activity relationships between, test materials.  
5.6 Results of acute toxicity tests will depend on the temperature, composition of the dilution water, condition of the test organisms, exposure technique, and other factors.
SCOPE
1.1 This guide (1)2 describes procedures for obtaining laboratory data concerning the adverse effects (for example, lethality and immobility) of a test material added to dilution water, but not to food, on certain species of freshwater and saltwater fishes, macroinvertebrates, and amphibians, usually during 2 to 4-day exposures, depending on the species. These procedures will probably be useful for conducting acute toxicity tests with many other aquatic species, although modifications might be necessary.  
1.2 Other modifications of these procedures might be justified by special needs or circumstances such as meeting specific study goals, regulatory needs, or to accommodate specific test organism life stages. Although using appropriate procedures is more important than following prescribed procedures, results of tests conducted using unusual or novel procedures are not likely to be comparable to results of many other tests. Comparison of results obtained using modified and unmodified versions of these procedures might provide useful information concerning new concepts and procedures for conducting acute tests.  
1.3 This guide describes tests using three basic exposure techniques: static, renewal, and flow-through. Selection of the technique to use in a specific situation will depend on the needs of the investigator and on available resources. Tests using the static technique provide the most easily obtained measure of acute toxicity, but conditions often change substantially during static tests; therefore, static tests should not last longer than 96 h, and test organisms should not be fed during such tests unless the test organisms are severely stressed without feeding over 48 h. Static tests should probably not be conducted on materials that have a high oxygen demand, are highly volatile, are rapidly transformed biologically or chemically in aqueous solution, or are removed from test solutions in substantial quantities by the test chambers or organisms during the test. Because the pH and concentrations of dissolved oxygen and test material are maintained at desired levels and degradation and metabolic products are removed, tests using ren...

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ASTM
ASTM E1242-23(Practice)
Standard Practice for Using Octanol-Water Partition Coefficient to Estimate Median Lethal Concentrations for Fish Due to Narcosis

SIGNIFICANCE AND USE
5.1 This procedure can be used to limit the need for screening tests prior to performing a test for estimating the LC50 of a non-reactive and non-electrolytic chemical to the fathead minnow. By eliminating the screening test, fewer fish need be tested. The time used for preparing and performing the screening test can also be saved. The value obtained in this procedure can be used as the preliminary estimate of the LC50 in a full-scale test.  
5.2 Estimates can be used to set testing priority of groups of non-reactive and non-electrolytic chemicals.  
5.3 If the estimated value is more than 0.3 times the experimental value, the mechanism of action is probably narcosis. If less, the effect concentration is considered to reflect a different mechanism of action.  
5.4 This practice estimates a maximum LC50, that is, non-reactive and non-electrolytic chemicals are at least as toxic as the practice predicts, but may have a lower LC50 if acting by a more specific mechanism. Data on a chemical indicating a lower toxicity than predicted should be considered suspect or an artifact because of limited solubility of the test material.
SCOPE
1.1 This practice covers a procedure for estimating the fathead minnow (Pimephales promelas) 96-h LC50 of nonreactive (that is, covalently bonded without unsaturated residues) and nonelectrolytic (that is, require vigorous reagents to facilitate substitution, addition, replacement reactions and are non-ionic, non-dissociating in aqueous solutions) organic chemicals acting solely by narcosis, also referred to as Meyer-Overton toxicity relationship.2  
1.2 This procedure is accurate for organic chemicals that are toxic due to narcosis and are non-reactive and non-electrolytic. Examples of appropriate chemicals are: alcohols, ketones, ethers, simple halogenated aliphatics, aromatics, and aliphatic substituted aromatics. It is not appropriate for chemicals whose structures include a potential toxiphore (that structural component of a chemical molecule that has been identified to show mammalian toxicity, for example CN is known to be reponsible for inactivation of enzymes, NO2 for decoupling of oxidative phosphorylation, both leading to mammalian toxicity). Examples of chemicals inappropriate for this practice are: carbamates, organophosphates, phenols, beta-gamma unsaturated alcohols, electrophiles, and quaternary ammonium salts.  
1.3 This international standard was developed in accordance with internationally recognized principles on standardization established in the Decision on Principles for the Development of International Standards, Guides and Recommendations issued by the World Trade Organization Technical Barriers to Trade (TBT) Committee.

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