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REACH

Nitrosodiphenylamine

EC number: 201-663-0 | CAS number: 86-30-6

Life Cycle description
Uses advised against

Toxicological information

Genetic toxicity: in vitro

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Administrative data

Endpoint:: in vitro gene mutation study in bacteria
Type of information:: experimental study
Adequacy of study:: weight of evidence
Reliability:: 2 (reliable with restrictions)
Rationale for reliability incl. deficiencies:: study well documented, meets generally accepted scientific principles, acceptable for assessment

Data source

Reference

Reference Type:: publication
Title:: Salmonella mutagenicity tests: IV Results from the testing of 300 chemicals
Author:: Zeiger E.
Year:: 1988
Bibliographic source:: Environ. Molecular mutagenesis Vol 11, suppl 12: 1-158

Materials and methods

Test guideline

Qualifier:: no guideline followed

Principles of method if other than guideline:: Test chemical was tested for mutagenicity in salmonella typhimurium, using a preincubation protocol. All tests were performed in the absence of exogenoux metabolic activation, and in the presenceof liver S-9 from Aroclor-induced male Sprague Dawley rats and Syrian hamsters.
GLP compliance:: no
Type of assay:: bacterial reverse mutation assay

Test material

Test material information

Constituent 1

Reference substance name:: Nitrosodiphenylamine
EC Number:: 201-663-0
EC Name:: Nitrosodiphenylamine
Cas Number:: 86-30-6
Molecular formula:: C12H10N2O
IUPAC Name:: N-nitroso-N-phenylaniline

Method

Species / strainopen all close all

Species / strain 1

Species / strain / cell type:: S. typhimurium TA 1535, TA 1537, TA 98 and TA 100
Additional strain / cell type characteristics:: not applicable

Species / strain 2

Species / strain / cell type:: S. typhimurium TA 97
Additional strain / cell type characteristics:: not applicable

Metabolic activation:: with and without
Metabolic activation system:: 10% or 30% of liver rat or hamster S9
Test concentrations with justification for top dose:: 0, 1000, 3300, 10000, 33000, 100000, 200000 µg/plate
Vehicle / solvent:: DMSO

Controls

Untreated negative controls:: yes
Negative solvent / vehicle controls:: yes
True negative controls:: no
Positive controls:: yes
Positive control substance:: 9-aminoacridine; sodium azide; other: 4-nitro-o-phenylenediamine (-S9, TA98)? 2-aminoanthracene (+S9, all strains)

Details on test system and experimental conditions:: Prepration of liver S9 fraction :
The S9 fractions of Aroclor 1254-induced, male SD rat ad male syrian hamster livers were prepared immediately prior to se and contained either 10% or 30% S9; occasionally, other levels were used. All chemicals were tested in the absence of metabolic activation, and with rat and hamster S9 fractions.

Test protocol :
The preincubation assay was performed as follow : the test chemical (0.05 ml), Salmonella culture (0.10 ml), and S9 mix or buffer (0.5 ml) were incubated at 37°C, without shaking for 20 min. The top agar was added and the contents of the tubes were mixed and poured onto the surfce of petri dishes containing medium. The histidine-independent (his +à colonies arising on these plates were counted following two days incubation at 37°C. Plates were machine counted unless precipitate was present which interfered with the count, or the color of the test chemical on the plate reduced the contrast between the colonies and the background agar. At the discretion of the investigators, plates with low numbers of colonies were counted by hand.
All chemicals were tested initially in a toxicity assay to determine the appropriate dose range for mutagnicity assay. The toxicity assay was performed using TA100. Toxic concentrations were those that produced a decrease in the number of his+ colonies, or a clearing in the density of the background lawn, or both.
Each chemical was tested initially at half-log dose intervals up to a dose that elicited toxicity, or to a dose immediately below one which was toxic in the preliminary test. Chemicals that were not toxic were tested to a miximum dose of 10 mg/plate. Chemicals that were poorly soluble were tested up to doses defined by their solubilities. At least 5 doses of each chemical were tested in triplicate. Experiments were repeated at least one week following the initial trial. A maximum of 0.05 ml solvent was added to each plate.
Evaluation criteria:: Evaluationswere made at both the individual trial and overall chemical levels. Individual triales were judged as mutegnic or not depending on the magnitude of the increase of his+ revertants, and the shape of the dose-response.
Statistics:: no

Results and discussion

Test results

Species / strain:: S. typhimurium, other: all strains
Metabolic activation:: with and without
Genotoxicity:: negative
Cytotoxicity / choice of top concentrations:: cytotoxicity
Vehicle controls validity:: valid
Untreated negative controls validity:: valid
Positive controls validity:: valid

Additional information on results:: see tables below