Evaluation of lymphocyte proliferation by immunohistochemistry in the local lymph node assay

Boussiquet-Leroux, Christine; Durand-Cavagna, G.; Herlin, K.; Holder, Daniel

doi:10.1002/jat.2550150608

Cited by 23 publications

(4 citation statements)

References 31 publications

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“…Flow cytometric analysis and immunohistochemical assays have been developed to count BrdU incorporation into lymph node cells (Boussiquet-Leroux et al, 1995;Lee et al, 2002, Suda et al, 2002. Takeyoshi et al (2001) investigated BrdU incorporation into lymph node cells by using a cell proliferation ELISA kit but their results for a number of allergens suggested an insufficient sensitivity because the increase in lymph node cell counts was not taken into account when calculating SI values (Takeyoshi et al, 2006).…”

Section: Discussionmentioning

confidence: 99%

Evaluation of auricular lymph node cell lymphocyte proliferation and cytokine production as non-radioactive endpoints during murine contact allergy

Ülker

Atak

Ateş

et al. 2011

Journal of Immunotoxicology

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Section: Discussionmentioning

confidence: 99%

Evaluation of auricular lymph node cell lymphocyte proliferation and cytokine production as non-radioactive endpoints during murine contact allergy

Ülker

Atak

Ateş

et al. 2011

Journal of Immunotoxicology

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“…(This was obtained with 20% Salicylic Acid.) Boussiquet-Leroux et al (1995) reported results of an LLNA performed using 5% to 20% Salicylic Acid dissolved 4:1 in acetone-olive oil (AOO). Groups of four female CD1 mice were dosed on the dorsum of the external ears with 25 µl of the test solution or the vehicle once daily on days 1 to 3.…”

Section: Salicylic Acidmentioning

confidence: 99%

Safety Assessment of Salicylic Acid, Butyloctyl Salicylate, Calcium Salicylate, C12–15 Alkyl Salicylate, Capryloyl Salicylic Acid, Hexyldodecyl Salicylate, Isocetyl Salicylate, Isodecyl Salicylate, Magnesium Salicylate, MEA-Salicylate, Ethylhexyl Salicylate, Potassium Salicylate, Methyl Salicylate, Myristyl Salicylate, Sodium Salicylate, TEA-Salicylate, and Tridecyl Salicylate

2003

Int J Toxicol

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Salicylic Acid is an aromatic acid used in cosmetic formulations as a denaturant, hair-conditioning agent, and skin-conditioning agent--miscellaneous in a wide range of cosmetic products at concentrations ranging from 0.0008% to 3%. The Calcium, Magnesium, and MEA salts are preservatives, and Potassium Salicylate is a cosmetic biocide and preservative, not currently in use. Sodium Salicylate is used as a denaturant and preservative (0.09% to 2%). The TEA salt of Salicylic Acid is used as an ultraviolet (UV) light absorber (0.0001% to 0.75%). Several Salicylic Acid esters are used as skin conditioning agents--miscellaneous (Capryloyl, 0.1% to 1%; C12-15 Alkyl, no current use; Isocetyl, 3% to 5%; Isodecyl, no current use; and Tridecyl, no current use). Butyloctyl Salicylate (0.5% to 5%) and Hexyldodecyl Salicylate (no current use) are hair-conditioning agents and skin-conditioning agents--miscellaneous. Ethylhexyl Salicylate (formerly known as Octyl Salicylate) is used as a fragrance ingredient, sunscreen agent, and UV light absorber (0.001% to 8%), and Methyl Salicylate is used as a denaturant and flavoring agent (0.0001% to 0.6%). Myristyl Salicylate has no reported function. Isodecyl Salicylate is used in three formulations, but no concentration of use information was reported. Salicylates are absorbed percutaneously. Around 10% of applied salicylates can remain in the skin. Salicylic Acid is reported to enhance percutaneous penetration of some agents (e.g., vitamin A), but not others (e.g., hydrocortisone). Little acute toxicity (LD(50) in rats; >2 g/kg) via a dermal exposure route is seen for Salicylic Acid, Methyl Salicylate, Tridecyl Salicylate, and Butyloctyl Salicylate. Short-term oral, inhalation, and parenteral exposures to salicylates sufficient to produce high blood concentrations are associated primarily with liver and kidney damage. Subchronic dermal exposures to undiluted Methyl Salicylate were associated with kidney damage. Chronic oral exposure to Methyl Salicylate produced bone lesions as a function of the level of exposure in 2-year rat studies; liver damage was seen in dogs exposed to 0.15 g/kg/day in one study; kidney and liver weight increases in another study at the same exposure; but no liver or kidney abnormalities in a study at 0.167 g/kg/day. Applications of Isodecyl, Tridecyl, and Butyloctyl Salicylate were not irritating to rabbit skin, whereas undiluted Ethylhexyl Salicylate produced minimal to mild irritation. Methyl Salicylate at a 1% concentration with a 70% ethanol vehicle were irritating, whereas a 6% concentration in polyethylene glycol produced little or no irritation. Isodecyl Salicylate, Methyl Salicylate, Ethylhexyl (Octyl) Salicylate, Tridecyl Salicylate, and Butyloctyl Salicylate were not ocular irritants. Although Salicylic Acid at a concentration of 20% in acetone was positive in the local lymph node assay, a concentration of 20% in acetone/olive oil was not. Methyl Salicylate was negative at concentrations up to 25% in this assay, independent of vehicle. Maximization te...

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“…To assess skin sensitization, murine local lymph node assays (LLNAs), which require relatively few animals in consideration of animal welfare, have been extensively used (Kimber and Weisenberger, ; OECD, ; Klink and Meade, ; Vandebriel et al , ). Although the standard LLNA endpoint is determination of the degree of 3 H‐methyl thymidine incorporation into lymphocytes (Boussiquet‐Leroux et al , ; Homey et al , ; Takeyoshi et al , ; Suda et al , ), alternative methods and endpoints have been used to reduce the number of animals or exclude the use of radioactivity. To this end, other clinical data, such as ear thickness, lymph node (LN) weight and cell counts, have been used as toxicological endpoints for assessment of chemical sensitizing potential (Homey et al , ; Vohr et al , ; Ehling et al , 2005a, b; Ku et al , ).…”

Section: Introductionmentioning

confidence: 99%

Pathway analysis of gene expression in local lymph nodes draining skin exposed to three different sensitizers

Jeong

Kang

et al. 2011

J of Applied Toxicology

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Genomic analysis in the local lymph node assays (LLNAs) is useful for assessing skin sensitization of chemicals and providing insights into mechanisms of sensitization. In this study, we collected 1406 genes from previous microarray findings, validated changes in their expression by RT-PCR analysis in local lymph nodes draining skin exposed to different sensitizers, and interpreted their biological function through pathway-based genomic analysis, in which 468 genes were identified as being in the KEGG pathway database. The top-ranked functions (P < 0.01) identified as being affected by the sensitizers were associated with aspects of cell growth, such as DNA replication, cell cycle regulation and pyrimidine metabolism. All the sensitizers tested (DNCB, OXA and TDI) induced significant up-regulation of Psme4, which is associated with DNA replication; Tfdp1, which is related to cell cycle regulation; and Dut, which is involved in pyrimidine metabolism. Specific changes were also shown in functional categories related to the immune response, including cytokines and their receptors. Genes identified in these functional categories, such as Ccl21c, Cxcl9, Cxcl10, Ifng and Il12rb1, were found to have functional relevance. These findings may enhance our understanding and assessment of chemical sensitizers, and enable us to distinguish sensitizers from irritants and to classify chemicals as contact sensitizers.

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Evaluation of lymphocyte proliferation by immunohistochemistry in the local lymph node assay

Cited by 23 publications

References 31 publications

Evaluation of auricular lymph node cell lymphocyte proliferation and cytokine production as non-radioactive endpoints during murine contact allergy

Evaluation of auricular lymph node cell lymphocyte proliferation and cytokine production as non-radioactive endpoints during murine contact allergy

Pathway analysis of gene expression in local lymph nodes draining skin exposed to three different sensitizers

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