TIME-RELATED DYNAMICS OF VARIATION IN CORE CLOCK GENE EXPRESSION LEVELS IN TISSUES RELEVANT TO THE IMMUNE SYSTEM

被引:24
|
作者
Mazzoccoli, G. [1 ,2 ,3 ]
Sothern, R. B. [4 ]
Greco, A. [3 ,5 ,6 ]
Pazienza, V. [3 ,7 ]
Vinciguerra, M. [8 ]
Liu, S. [9 ]
Cai, Y. [9 ]
机构
[1] Inst Sci, Dept Internal Med, San Giovanni Rotondo, FG, Italy
[2] Inst Sci, Chronobiol Unit, San Giovanni Rotondo, FG, Italy
[3] Reg Gen Hosp Casa Sollievo Sofferenza, San Giovanni Rotondo, FG, Italy
[4] Univ Minnesota, Coll Biol Sci, Ctr Biol Sci, Rhythmometry Lab, St Paul, MN 55108 USA
[5] Inst Sci, Dept Med Sci, Geriatr Unit, San Giovanni Rotondo, FG, Italy
[6] Inst Sci, Dept Med Sci, Gerontol Geriatr Res Lab, San Giovanni Rotondo, FG, Italy
[7] Inst Sci, Gastroenterol Unit, Res Lab, San Giovanni Rotondo, FG, Italy
[8] Birkbeck Coll, Inst Hepatol, London, England
[9] Capital Med Univ, Xuanwu Hosp, Dept Neurol & Neurobiol, Key Lab Neurodegenerat Dis,Minist Educ, Beijing, Peoples R China
关键词
clock gene; circadian rhythm; immune system; CIRCADIAN-RHYTHMS; LYMPHOCYTE SUBPOPULATIONS; TRANSCRIPTION; LEUKOCYTES; RESPONSES; CORTISOL; HEALTH; BMAL1; GAMMA;
D O I
10.1177/039463201102400406
中图分类号
R392 [医学免疫学]; Q939.91 [免疫学];
学科分类号
100102 ;
摘要
Immune parameters show rhythmic changes with a 24-h periodicity driven by an internal circadian timing system that relies on clock genes (CGs). CGs form interlocked transcription-translation feedback loops to generate and maintain 24-h mRNA and protein oscillations. In this study we evaluate and compare the profiles and the dynamics of variation of CG expression in peripheral blood, and two lymphoid tissues of mice. Expression levels of seven recognized key CGs (mBmal1, mClock, mPer1, mPer2, mCry1, mCry2, and Rev-erb alpha) were evaluated by quantitative RT-PCR in spleen, thymus and peripheral blood of C57BL/6 male mice housed on a 12-h light (L)-dark (D) cycle and sacrificed every 4 h for 24 h (3-4 mice/time point). We found a statistically significant time-effect in spleen (S), thymus (T) and blood (B) for the original values of expression level of mBmal1 (S), mClock (T, B), mPer1 (S, B), mPer2 (S), mCry1 (S), mCry2 (B) and mRev-Erb alpha (S, T, B) and for the fractional variation calculated between single time-point expression value of mBmal1 (B), mPer2 (T), mCry2 (B) and mRev-Erb alpha (S). A significant 24-h rhythm was validated for five CGs in blood (mClock, mPer1, mPer2, mCry2, mRevErb alpha), for four CGs in the spleen (mBmal1, mPerl, mPer2, mRev-Erb alpha), and for three CGs in the thymus (mClock, mPer2, mRev-Erb alpha). The original values of acrophases for mBmal1, mClock, mPerl, mPer2, mCry1 and mCry2 were very similar for spleen and thymus and advanced by several hours for peripheral blood compared to the lymphoid tissues, whereas the phases of mRev-Erb alpha were coincident for all three tissues. In conclusion, central and peripheral lymphoid tissues in the mouse show different sequences of activation of clock gene expression compared to peripheral blood. These differences may underlie the compartmental pattern of web functioning in the immune system.
引用
收藏
页码:869 / 879
页数:11
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