Abstract

The overall goal of this research will be to understand the fundamental mechanisms by which trichothecene mycotoxins target leukocytes and dysregulate immune function. The trichothecene mycotoxins are common food and indoor air contaminants that have been etiologically linked to human and animal disease. In experimental animals, how level trichothecene exposure evokes upregulated cytokine production with attendant autoimmune sequelae, whereas exposure to higher levels induces leukocyte apoptosis with accompanying immune suppression. Upon examining upstream events that may contribute to these divergent effects, it was observed that mitogen-activated kinases (MAPKs) JNK 1 / 2, ERK 1 / 2, and p38 are rapidly and variably phosphorylated following exposure to trichothecenes in vitro and in vivo. Based on these findings and known downstream functions of these kinases, it is hypothesized that immune stimulation and suppression by trichothecenes are mediated by differential activation of MAPK, signaling cascades. Three SPECFIC AIMS are proposed to test this hypothesis.
In Aim 1, trichothecene-mediated activation of specific MAPKs will be related to changes in transcriptional and post-transcriptional regulation of cytokine gene expression in RAW 264.7 cells, a cloned macrophage model. To define contributions of specific MAPKs, the effects of selectively impairing JNK 1 / 2, ERK 1 / 2, and p38 function/expression by pharmacologic and genetic means on regulation of cytokine expression will be measured.
In Aim 2, trichothecene-medicated activation of specific MAPKs will be related to apoptosis in RAW 264.7 cells. The contributions of p53 activation and expression of downstream apoptotic effectors Bax, Bcl-XI and caspase-3 in trichothecene-induced apoptosis will be assessed. The effects of selectively blocking JNK 1 / 2, ERK 1 / 2, and p38 function/expression on regulation of the apoptotic pathway will be determined.
In Aim 3, putative mechanisms will be further verified in mice orally exposed to trichothecenes by qualifying the effects of trichothecene dose and exposure time on MAPK phosphorylation/activation and relating these to regulation of cytokine mRNA expression and apoptosis in lymphoid tissues. The sensitivity of various tissues and leukocyte phenotypes to trichothecene-induced MAPK phosphorylation will be compared. The effects of selectively inhibiting JNK 1 / 2, ERK 1 / 2 and p38 in vivo and ex vivo on cytokine mRNA expression and apoptosis will be addressed. Over the long term, this research will help characterize hazards associated with trichothecene exposure that can be used in human risk assessment.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Institute of Environmental Health Sciences (NIEHS)
Type
Research Project (R01)
Project #
5R01ES003358-17
Application #
6518029
Study Section
Alcohol and Toxicology Subcommittee 4 (ALTX)
Program Officer
Heindel, Jerrold
Project Start
1984-03-01
Project End
2005-03-31
Budget Start
2002-04-01
Budget End
2003-03-31
Support Year
17
Fiscal Year
2002
Total Cost
$260,677
Indirect Cost

  Institution

Name
Michigan State University
Department
Nutrition
Type
Schools of Earth Sciences/Natur
DUNS #
193247145
City
East Lansing
State
MI
Country
United States
Zip Code
48824

  Publications

Pestka, James J; Clark, Erica S; Schwartz-Zimmermann, Heidi E et al. (2017) Sex Is a Determinant for Deoxynivalenol Metabolism and Elimination in the Mouse. Toxins (Basel) 9:
Wu, Wenda; Zhou, Hui-Ren; Bursian, Steven J et al. (2016) Emetic responses to T-2 toxin, HT-2 toxin and emetine correspond to plasma elevations of peptide YY3-36 and 5-hydroxytryptamine. Arch Toxicol 90:997-1007
Wu, Wenda; Zhou, Hui-Ren; Pan, Xiao et al. (2015) Comparison of Anorectic Potencies of the Trichothecenes T-2 Toxin, HT-2 Toxin and Satratoxin G to the Ipecac Alkaloid Emetine. Toxicol Rep 2:238-251
Clark, Erica S; Flannery, Brenna M; Pestka, James J (2015) Murine Anorectic Response to Deoxynivalenol (Vomitoxin) Is Sex-Dependent. Toxins (Basel) 7:2845-59
Clark, Erica S; Flannery, Brenna M; Gardner, Elizabeth M et al. (2015) High Sensitivity of Aged Mice to Deoxynivalenol (Vomitoxin)-Induced Anorexia Corresponds to Elevated Proinflammatory Cytokine and Satiety Hormone Responses. Toxins (Basel) 7:4199-215
Zhou, Hui-Ren; Pestka, James J (2015) Deoxynivalenol (Vomitoxin)-Induced Cholecystokinin and Glucagon-Like Peptide-1 Release in the STC-1 Enteroendocrine Cell Model Is Mediated by Calcium-Sensing Receptor and Transient Receptor Potential Ankyrin-1 Channel. Toxicol Sci 145:407-17
Wu, Wenda; He, Kaiyu; Zhou, Hui-Ren et al. (2014) Effects of oral exposure to naturally-occurring and synthetic deoxynivalenol congeners on proinflammatory cytokine and chemokine mRNA expression in the mouse. Toxicol Appl Pharmacol 278:107-15
Pan, Xiao; Whitten, Douglas A; Wilkerson, Curtis G et al. (2014) Dynamic changes in ribosome-associated proteome and phosphoproteome during deoxynivalenol-induced translation inhibition and ribotoxic stress. Toxicol Sci 138:217-33
Pan, Xiao; Whitten, Douglas A; Wu, Ming et al. (2013) Early phosphoproteomic changes in the mouse spleen during deoxynivalenol-induced ribotoxic stress. Toxicol Sci 135:129-43
He, Kaiyu; Pan, Xiao; Zhou, Hui-Ren et al. (2013) Modulation of inflammatory gene expression by the ribotoxin deoxynivalenol involves coordinate regulation of the transcriptome and translatome. Toxicol Sci 131:153-63

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