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Nanotechnologies -- 5-(and 6)-Chloromethyl-2', 7' Dichloro-dihydrofluorescein diacetate (CM-H2DCF-DA) assay for evaluating nanoparticle-induced intracellular reactive oxygen species(ROS) production in RAW 264.7 macrophage cell line
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Basic data | Standard ID | GB/T 41212-2021 (GB/T41212-2021) | | Description (Translated English) | Nanotechnologies -- 5-(and 6)-Chloromethyl-2', 7' Dichloro-dihydrofluorescein diacetate (CM-H2DCF-DA) assay for evaluating nanoparticle-induced intracellular reactive oxygen species(ROS) production in RAW 264.7 macrophage cell line | | Sector / Industry | National Standard (Recommended) | | Classification of Chinese Standard | C04 | | Word Count Estimation | 22,220 | | Issuing agency(ies) | State Administration for Market Regulation, China National Standardization Administration |
GB/T 41212-2021: Nanotechnologies -- 5-(and 6)-Chloromethyl-2', 7' Dichloro-dihydrofluorescein diacetate (CM-H2DCF-DA) assay for evaluating nanoparticle-induced intracellular reactive oxygen species(ROS) production in RAW 264.7 macrophage cell line
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Nanotechnologies -- 5-(and 6)-Chloromethyl-2', 7' Dichloro-dihydrofluorescein diacetate (CM-H2DCF-DA) assay for evaluating nanoparticle-induced intracellular reactive oxygen species(ROS) production in RAW 264:7 macrophage cell line
ICS 07:120
CCSC04
National Standards of People's Republic of China
Nanotechnology Fluorescein Diacetate Detection
Nanoparticle-induced production of reactive oxygen species in macrophages
(ISO /T S19006:2016, IDT)
Published on 2021-12-31
2022-07-01 Implementation
State Administration for Market Regulation
Released by the National Standardization Administration
directory
Preface I
Introduction II
1 Scope 1
2 Normative references 1
3 Terms and Definitions 1
4 Symbols and Abbreviations 3
5 Material 3
6 Technical equipment 4
7 Nanoparticle sample preparation 4
8 Preparation 5
8:1 Overview 5
8:2 Flow Cytometry Calibration 6
8:3 Experimental Medium 6
8:4 Reagent preparation 6
8:5 Preparation of cell cultures 6
8:6 Preparing cultures for experiments 6
8:7 Detection of cell growth status 6
8:8 Evaluating Nanoparticle Interference 7
8:9 Preparation of the control group 8
8:9:1 Overview 8
8:9:2 Description of the control group 8
8:9:3 Sin-1 stock solution preparation (1 mM) 8
9 Evaluating the effect of nanomaterials on intracellular ROS production 8
9:1 Preparation of cells in 24-well plates 8
9:2 Treatment of cells with controls and different concentrations of nanoparticles 8
9:3 Exposure of CM-H2DCF-DA cells 9
9:4 Incubation of cells with CM-H2DCF-DA 9
9:5 Flow Cytometry Analysis 9
10 Data Analysis and Results 10
Appendix A (Informative) Alternative Cell Lines 11
Appendix B (Informative) Alternative Fluorescence Characterization Techniques 12
Appendix C (Informative) Preparation and Characterization of Suspensions 13
Appendix D (Informative) Example 14 of Experimental Data from RAW264:7
Reference 16
foreword
This document is in accordance with the provisions of GB/T 1:1-2020 "Guidelines for Standardization Work Part 1: Structure and Drafting Rules of Standardization Documents"
drafted:
This document uses the translation method equivalent to ISO /T S19006:2016 "Nanotechnology Fluorescein Diacetate Method for the Detection of Nanoparticle Inducements"
Reactive Oxygen Species Produced by Macrophages":
The Chinese documents that have a consistent correspondence with the international documents normatively cited in this document are as follows:
---GB/T 16886:5-2017 Biological Evaluation of Medical Devices Part 5: In Vitro Cytotoxicity Test (ISO 10993-5:
2009, IDT):
The following editorial changes have been made to this document:
--- The documents cited in the introductory phrase of the Chapter Terms and Definitions are listed in Chapter 2 "Normative Reference Documents";
--- References reordered:
Please note that some content of this document may be patented: The issuing agency of this document assumes no responsibility for identifying patents:
This document is proposed by the Chinese Academy of Sciences:
This document is under the jurisdiction of the National Nanotechnology Standardization Technical Committee (SAC/TC279):
This document was drafted by: National Nanoscience Center, Institute of Basic Medicine, Chinese Academy of Medical Sciences, China National Institute for Food and Drug Control:
The main drafters of this document: Wu Xiaochun, Ji Yinglu, Fan Huizhen, Li Haiyun, Li Yiye, Nie Guangjun, Xu Haiyan, Wen Tao, Wen Hairuo, Danmo:
Introduction
With the continuous development of new materials, products and applications, the field of nanotechnology continues to develop rapidly: At the same time, some of the
Concerns about potential risks to human health and the environment posed by rice-based materials are also on the rise: At present, a large number of related researches are being carried out internationally
research to better understand and quantify these potential risks: In addition, the coatings used to coat the surface of nanoparticles during processing or in the final product
Chemicals may also affect the interaction between nanoparticles and cells: Especially considering the large specific surface area of nanoparticles, this
The impact may be more pronounced: Therefore, it is necessary to develop reliable and rapid screening methods for these chemically functionalized nanoparticles:
Potential particle toxicity:
Monitoring the biological response of model cells after nanoparticle exposure promises to deepen our understanding of the nanoparticle "mode of action", and to judge
Which of these factors may require further study for subsequent risk assessment:
In:2008, some international research teams found that some published nanomaterial toxicity research results could not be replicated in different laboratories:
Therefore, there is a need to develop accurate and reproducible nanotoxicological testing methods: International Consortium for Nano Environmental Health and Safety (nanoEHS) Coordination
(IANH) came into being to develop test protocols that can accurately assess nanoparticle toxicity and its biological effects on cells, and these tests
The test procedure can be repeated in any laboratory: IANH adopts 3-(4,5-dimethylthiazol-2-yl)-5-(3-carboxymethoxyphenyl)-2-(4-sulfonic acid)
phenyl)-2H-tetrazole (MTS) method, 5-(6)-chloromethyl-2',7'-dichloro-dihydrofluorescein diacetate (CM-H2DCF-DA) method and Iodine
The propidium method was used to compare the particle size distribution in liquid suspension and the in vitro interaction of nanomaterials with cells: IANH Discovery
Some factors that increase test uncertainty have been identified, and techniques have been developed to reduce such uncertainty:
Oxidative stress can lead to DNA damage and is the main driving force for the accumulation of mutations in organisms: Therefore, it was assessed whether the nanoparticles would lead to
It is very important to activate cells to produce reactive oxygen species (ROS):
This document provides an in vitro measurement to assess ROS production from cellular exposure to nanoparticles: Although measuring intracellular ROS production has
There are many techniques, but only the CM-H2DCF-DA method has been carried out to evaluate the ROS production of RAW264:7 mouse macrophages:
The CM-H2DCF-DA method is a common method to detect cellular oxidative stress, which is not specific for oxygen free radicals or oxygen-reactive species [9]:
Although this method has not been evaluated in a wider range of cell lines, it provides insight into the possibility of ROS production in macrophages,
This mechanism may play an important role in clearing particles from the body:
In the presence of a control group, the CM-H2DCF-DA method may also be misjudged: Several factors may contribute to false negatives [9]:
The CM-H2DCF-DA method does not achieve optimal detection for all ROS: For example, for the short half-life superoxide anion and hydroxyl
Free radicals, its detection effect is not good: 2',7'-Dichlorodihydrofluorescein (DCFH) and 2',7'-Dichlorofluorescein (DCF) can be leached from cells
Or DCFH is oxidized, so when measured by flow cytometry, it should be detected quickly after cell exposure: In addition, the CM-H2DCF-DA method
Ineffective in serum, the process of washing cells to remove serum may cause cell loss, resulting in false negatives: Some nanoparticles may be associated with
The DCFH interaction results in partial quenching of fluorescence: Therefore, if the above conditions exist, the negative results of ROS measured by the experiment are not absolute:
of: ISO /T S18827 detects ROS in cells by electron spin resonance (ESR) spectroscopy: This method can be used without interference
Divide into different ROS:
In turn, some factors may cause false positives [10]: Some nanoparticles and dead cells fluoresce: Some nanoparticles can catalyze
CM-H2DCF-DA oxidation: Detection reagents may be preferentially adsorbed on the particle surface [10]: To ensure that positive results are reliable, the test conditions should be
The control group was used to characterize the nanoparticles alone, and to distinguish the fluorescence produced by dead cells from the fluorescence produced by ROS in living cells:
In addition, CM-H2DCF-DA can undergo light-induced auto-oxidation, so its stock solution should be kept in a nitrogen/argon-filled airtight solution regardless of its concentration:
Store in a closed container away from light to prevent light and air from entering:
Therefore, the CM-H2DCF-DA method may only be applicable to specific cell lines and nanoparticles: Before drawing a final conclusion, it should also be
Additional assays provide further confirmation of the results (see Appendix A for Alternative Cell Lines): When the detection system has the potential to cause false
This is especially important when considering factors for negative or false-positive results: For example, for a positive result, other tests should be found to ensure that the positive result
If not caused by interference: Other factors to consider include: a control group should be used to determine the baseline fluorescence of unexposed cells; cells should be determined
Is it affected by non-toxic nanoparticles; it should be ensured that the ROS positive control reagent and the ROS generated by the nanoparticles are in the assay conditions used
can be detected below: In addition, it remains to be determined whether the nanoparticles interfere with the fluorescence assay, which further contributes to the particle-induced cellular ROS production:
The evaluation result is invalid: If this interference is possible, different doses of sodium can be added to cells exposed to 3-morpholinodiimide (Sin-1):
Control experiments were performed on rice particles to determine whether the nanoparticles quenched fluorescence:
NOTE: This method is considered to be a rapid screening method for nanoparticle-cell interactions: Although screening-like methods are used to assess the cellular effects of nanoparticles
This is critical, but it is also important that the interpretation of the results can be validated by other ROS and related cellular assays:
Nanotechnology Fluorescein Diacetate Detection
Nanoparticle-induced production of reactive oxygen species in macrophages
1 Scope
This document describes how 5-(6)-chloromethyl-2',7'dichlorodihydro-fluorescein diacetate (CM-H2DCF-DA) was detected and evaluated
Methods for the production of reactive oxygen species (ROS) after exposure of RAW264:7 macrophages to nanoobjects, nanoparticles and their aggregates and aggregates:
This document applies to assays using 24-well plates: If other well plates are used, adjust the sample volume and verify the effectiveness of the procedure to
Ensure that test results are credible:
2 Normative references
The contents of the following documents constitute essential provisions of this document through normative references in the text: Among them, dated citations
documents, only the version corresponding to that date applies to this document; for undated references, the latest edition (including all amendments) applies to
this document:
ISO 10993-5 Biological evaluation of medical devices - Part 5: In vitro cytotoxicity test (Biological evaluation of
medicaldevices-Part 5:Testsforinvitrocytotoxicity)
ISO /T S80004-2 Nanotechnology terminology Part 2: Nano-objects (Nanotechnologies-Vocabulary-Part 2:
Nano-objects)
3 Terms and Definitions
Terms and definitions defined in ISO /T S80004-2, ISO 10993-5 and the following apply to this document:
The following URLs are ISO and IEC responsible for database URLs used in standards:
ISO Online Browsing Platform: http://www:iso:org/obp
IEC online browsing platform: http://www:electropedia:org/
3:1
agglomerate
Stacks, aggregates or mixtures of weakly bound particles whose external surface area is similar to the sum of the surface areas of their individual particles:
Note 1: The forces supporting the aggregates are weak forces, such as van der Waals forces or simple physical entanglement:
Note 2: Aggregates are also referred to as secondary particles, while source particles are referred to as primary particles:
[Source: ISO /T S80004-2:2015, 3:4]
3:2
aggregate aggregate
New particles composed of strongly bound or fused particles may have an external surface area significantly smaller than the sum of their individual particle surface areas:
Note 1: The forces supporting the aggregates are strong forces, such as covalent bonds or originating from sintering or complex physical entanglement:
Note 2: Aggregates are also referred to as secondary particles, while source particles are referred to as primary particles:
[Source: ISO /T S80004-2:2015, 3:5]
3:3
culture vessel culturevessels
Including glass culture dishes, plastic culture flasks or plastic multi-well culture plates and microtiter plates and other vessels suitable for cell culture:
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