Your search keyword '"Kolle SN"' showing total 3 results

1. Immunophenotyping does not improve predictivity of the local lymph node assay in mice.

Author

Strauss V, Kolle SN, Honarvar N, Dammann M, Groeters S, Faulhammer F, Landsiedel R, and van Ravenzwaay B

Subjects

Animals, Antigens, Surface metabolism, Dermatitis, Contact immunology, Dermatitis, Contact metabolism, Female, Immunophenotyping, Local Lymph Node Assay, Lymph Nodes immunology, Lymph Nodes metabolism, Lymphocytes immunology, Lymphocytes metabolism, Mice, Inbred CBA, Surface-Active Agents chemistry, Haptens toxicity, Irritants toxicity, Lymph Nodes drug effects, Lymphocytes drug effects, Models, Biological

Abstract

The local lymph node assay (LLNA) is a regulatory accepted test for the identification of skin sensitizing substances by measuring radioactive thymidine incorporation into the lymph node. However, there is evidence that LLNA is overestimating the sensitization potential of certain substance classes in particular those exerting skin irritation. Some reports describe the additional use of flow cytometry-based immunophenotyping to better discriminate irritants from sensitizing irritants in LLNA. In the present study, the 22 performance standards plus 8 surfactants were assessed using the radioactive LLNA method. In addition, lymph node cells were immunophenotyped to evaluate the specificity of the lymph node response using cell surface markers such as B220 or CD19, CD3, CD4, CD8, I-A(κ) and CD69 with the aim to allow a better discrimination above all between irritants and sensitizers, but also non-irritating sensitizers and non-sensitizers. However, the markers assessed in this study do not sufficiently differentiate between irritants and irritant sensitizers and therefore did not improve the predictive capacity of the LLNA., (Copyright © 2014 John Wiley & Sons, Ltd.)

Published

2015

2. Further experience with the local lymph node assay using standard radioactive and nonradioactive cell count measurements.

Author

Kolle SN, Basketter D, Schrage A, Gamer AO, van Ravenzwaay B, and Landsiedel R

Subjects

Animals, Cell Count standards, Dermatitis, Allergic Contact metabolism, Disease Models, Animal, Dose-Response Relationship, Radiation, Female, Linear Models, Mice, Mice, Inbred CBA, Biological Assay methods, Biological Assay standards, Dermatitis, Allergic Contact pathology, Local Lymph Node Assay

Abstract

In a previous study, the predictive capacity of a modified local lymph node assay (LLNA) based on cell counts, the LNCC, was demonstrated to be closely similar to that of the original assay. In addition, a range of substances, including some technical/commercial materials and a range of agrochemical formulations (n = 180) have also been assessed in both methods in parallel. The results in the LNCC and LLNA were generally consistent, with 86% yielding an identical classification outcome. Discordant results were associated with borderline data and were evenly distributed between the two methods. Potency information derived from each method also demonstrated good consistency (n = 101), with 93% of predictions being close. Skin irritation was observed only infrequently and was most commonly associated with positive results; it was not associated with the discordant results. Where different vehicles were used with the same test material, the effect on sensitizing activity was modest, consistent with historical data. Analysis of positive control data indicated that the LNCC and LLNA displayed similar levels of biological variation. When taken in combination with the previously published results on LLNA Performance Standard chemicals, it is concluded that the LNCC provides a viable non-radioactive alternative to the LLNA for the assessment of substances, including potency predictions, as well as for the evaluation of preparations., (Copyright © 2012 John Wiley & Sons, Ltd.)

Published

2012

3. Experience with local lymph node assay performance standards using standard radioactivity and nonradioactive cell count measurements.

Author

Basketter D, Kolle SN, Schrage A, Honarvar N, Gamer AO, van Ravenzwaay B, and Landsiedel R

Subjects

Animals, Cell Count standards, Chlorobenzenes adverse effects, Chlorobenzenes analysis, Dermatitis, Allergic Contact metabolism, Endpoint Determination, Female, Linear Models, Methylmethacrylate adverse effects, Methylmethacrylate analysis, Mice, Mice, Inbred CBA, Nickel adverse effects, Nickel analysis, Radioactivity, Salicylates adverse effects, Salicylates analysis, Biological Assay methods, Biological Assay standards, Dermatitis, Allergic Contact pathology, Local Lymph Node Assay

Abstract

The local lymph node assay (LLNA) is the preferred test for identification of skin-sensitizing substances by measuring radioactive thymidine incorporation into the lymph node. To facilitate acceptance of nonradioactive variants, validation authorities have published harmonized minimum performance standards (PS) that the alternative endpoint assay must meet. In the present work, these standards were applied to a variant of the LLNA based on lymph node cell counts (LNCC) run in parallel as a control with the standard LLNA with radioactivity measurements, with threshold concentrations (EC3) being determined for the sensitizers. Of the 22 PS chemicals tested in this study, 21 yielded the same results from standard radioactivity and cell count measurements; only 2-mercaptobenzothiazole was positive by LLNA but negative by LNCC. Of the 16 PS positives, 15 were positive by LLNA and 14 by LNCC; methylmethacrylate was not identified as sensitizer by either of the measurements. Two of the six PS negatives tested negative in our study by both LLNA and LNCC. Of the four PS negatives which were positive in our study, chlorobenzene and methyl salicylate were tested at higher concentrations than the published PS, whereas the corresponding concentrations resulted in consistent negative results. Methylmethacrylate and nickel chloride tested positive within the concentration range used for the published PS. The results indicate cell counts and radioactive measurements are in good accordance within the same LLNA using the 22 PS test substances. Comparisons with the published PS results may, however, require balanced analysis rather than a simple checklist approach., (Copyright © 2011 John Wiley & Sons, Ltd.)

Published

2012