TY - JOUR
T1 - Germ-Free Conditions Modulate Host Purine Metabolism, Exacerbating Adenine-Induced Kidney Damage
AU - Mishima, Eikan
AU - Ichijo, Mariko
AU - Kawabe, Takeshi
AU - Kikuchi, Koichi
AU - Akiyama, Yukako
AU - Toyohara, Takafumi
AU - Suzuki, Takehiro
AU - Suzuki, Chitose
AU - Asao, Atsuko
AU - Ishii, Naoto
AU - Fukuda, Shinji
AU - Abe, Takaaki
N1 - Funding Information:
Funding: This study was supported in part by Grant-in-Aid for Scientific Research (18K08198 to E.M.) from the Japan Society for the Promotion of Science (JSPS), AMED-CREST (JP19gm1010009 to S.F.), JST ERATO (JPMJER1902 to S.F.), the Takeda Science Foundation (to S.F.), the Food Science Institute Foundation (to S.F.), the Program for the Advancement of Research in Core Projects under Keio University’s Longevity Initiative (to S.F.), a grant from the Japan Foundation for Applied Enzymology (to E.M), The Japan Health Foundation (to E.M), HIROMI Medical Research Foundation (to E.M), Okinaka Memorial Institute for Medical Research Grant (to E.M), and Tohoku University Center for Gender Equality Promotion (TUMUG) Support Project (to E.M).
Funding Information:
This study was supported in part by Grant-in-Aid for Scientific Research (18K08198 to E.M.) from the Japan Society for the Promotion of Science (JSPS), AMED-CREST (JP19gm1010009 to S.F.), JST ERATO (JPMJER1902 to S.F.), the Takeda Science Foundation (to S.F.), the Food Science Institute Foundation (to S.F.), the Program for the Advancement of Research in Core Projects under Keio University?s Longevity Initiative (to S.F.), a grant from the Japan Foundation for Applied Enzymology (to E.M), The Japan Health Foundation (to E.M), HIROMI Medical Research Foundation (to E.M), Okinaka Memorial Institute for Medical Research Grant (to E.M), and Tohoku University Center for Gender Equality Promotion (TUMUG) Support Project (to E.M). We acknowledge the support of Biomedical Research Core of Tohoku University Graduate School of Medicine. The images in Figure 7 were obtained from DBCLS Togo Picture Gallery (TogoTV; http: //togotv.dbcls.jp/ja/), PIXTA (https://pixta.jp/), and iStock (https://www.istockphoto.com/). We thank Y. Sasaki for technical assistance.
PY - 2020/9
Y1 - 2020/9
N2 - Alterations in microbiota are known to affect kidney disease conditions. We have previously shown that germ-free conditions exacerbated adenine-induced kidney damage in mice; however, the mechanism by which this occurs has not been elucidated. To explore this mechanism, we examined the influence of germ-free conditions on purine metabolism and renal immune responses involved in the kidney damage. Germ-free mice showed higher expression levels of purine-metabolizing enzymes such as xanthine dehydrogenase, which converts adenine to a nephrotoxic byproduct 2,8-dihydroxyadenine (2,8-DHA). The germ-free mice also showed increased urinary excretion of allantoin, indicating enhanced purine metabolism. Metabolome analysis demonstrated marked differences in the purine metabolite levels in the feces of germ-free mice and mice with microbiota. Furthermore, unlike the germ-free condition, antibiotic treatment did not increase the expression of purine-metabolizing enzymes or exacerbate adenine-induced kidney damage. Considering renal immune responses, the germ-free mice displayed an absence of renal IL-17A expression. However, the adenine-induced kidney damage in wild-type mice was comparable to that in IL-17A-deficient mice, suggesting that IL-17A does not play a major role in the disease condition. Our results suggest that the enhanced host purine metabolism in the germ-free mice potentially promotes the conversion of the administered adenine into 2,8-DHA, resulting in exacerbated kidney damage. This further suggests a role of the microbiota in regulating host purine metabolism.
AB - Alterations in microbiota are known to affect kidney disease conditions. We have previously shown that germ-free conditions exacerbated adenine-induced kidney damage in mice; however, the mechanism by which this occurs has not been elucidated. To explore this mechanism, we examined the influence of germ-free conditions on purine metabolism and renal immune responses involved in the kidney damage. Germ-free mice showed higher expression levels of purine-metabolizing enzymes such as xanthine dehydrogenase, which converts adenine to a nephrotoxic byproduct 2,8-dihydroxyadenine (2,8-DHA). The germ-free mice also showed increased urinary excretion of allantoin, indicating enhanced purine metabolism. Metabolome analysis demonstrated marked differences in the purine metabolite levels in the feces of germ-free mice and mice with microbiota. Furthermore, unlike the germ-free condition, antibiotic treatment did not increase the expression of purine-metabolizing enzymes or exacerbate adenine-induced kidney damage. Considering renal immune responses, the germ-free mice displayed an absence of renal IL-17A expression. However, the adenine-induced kidney damage in wild-type mice was comparable to that in IL-17A-deficient mice, suggesting that IL-17A does not play a major role in the disease condition. Our results suggest that the enhanced host purine metabolism in the germ-free mice potentially promotes the conversion of the administered adenine into 2,8-DHA, resulting in exacerbated kidney damage. This further suggests a role of the microbiota in regulating host purine metabolism.
KW - Chronic kidney disease
KW - Gut-kidney axis
KW - IL-17
KW - Microbiota
KW - Th17
KW - Uremic toxins
KW - Uric acids
KW - Xanthine dehydrogenase
KW - Xanthine oxidase
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U2 - 10.3390/toxins12090547
DO - 10.3390/toxins12090547
M3 - Article
C2 - 32859011
AN - SCOPUS:85090175353
VL - 12
JO - Toxins
JF - Toxins
SN - 2072-6651
IS - 9
M1 - 547
ER -