DISTRIBUTION OF ERYTHROPOIETIN PRODUCING CELLS IN RAT KIDNEYS DURING HYPOXIC HYPOXIA

被引:86
作者
ECKARDT, KU
KOURY, ST
TAN, CC
SCHUSTER, SJ
KAISSLING, B
RATCLIFFE, PJ
KURTZ, A
机构
[1] VANDERBILT UNIV, MED CTR, SCH MED, DEPT MED, DIV HEMATOL, NASHVILLE, TN 37232 USA
[2] JOHN RADCLIFFE HOSP, INST MOLEC MED, OXFORD OX3 9DU, ENGLAND
[3] THOMAS JEFFERSON UNIV, CARDEZA FDN HEMATOL RES, PHILADELPHIA, PA 19107 USA
[4] UNIV ZURICH, INST ANAT, CH-8006 ZURICH, SWITZERLAND
关键词
D O I
10.1038/ki.1993.115
中图分类号
R5 [内科学]; R69 [泌尿科学(泌尿生殖系疾病)];
学科分类号
1002 ; 100201 ;
摘要
We have used in situ hybridization to determine the localization and distribution of cells expressing the erythropoietin (EPO) gene in kidneys of rats exposed to reduced oxygen tensions to characterize the control of renal EPO formation during hypoxic hypoxia. Animals were subjected to severe hypoxia (7.5% O2) for 4, 8 and 32 hours to assess changes related to the duration of hypoxic exposure, and additionally to 9% and 11.5% O2 for eight hours to define changes related to the degree of hypoxia. The number of cells containing EPO mRNA were counted on tissue sections and compared to tissue concentrations of EPO mRNA and to the serum hormone concentrations. In situ hybridization revealed expression of the EPO gene exclusively in peritubular cells that were predominantly located in the cortical labyrinth under all conditions tested. After four hours of severe hypoxia (7.5% O2) approximately 170-fold more cells were found to contain EPO mRNA than under normoxic conditions. The number of EPO producing cells did not change significantly between four and eight hours exposure to 7.5% O2, but the amount of EPO mRNA per kidney increased approximately threefold. Further continuation of hypoxia resulted in down-regulation of renal EPO mRNA levels, which was mainly due to a reduction in the number of cells containing EPO mRNA. Comparison of graded degrees of hypoxia applied for eight hours showed an inverse exponential relationship between oxygen tension and the number of EPO producing cells. This recruitment of cells expressing the EPO gene occurred along a gradient extending from the corticomedullary border to the subcapsular tissue. In view of previous observations in anemic animals these findings indicate that the control of EPO formation under anemic and hypoxic hypoxia is similar. The cell type producing EPO appears to be identical and the number of cells expressing the EPO gene appears to be a major determinant of EPO production rate under both conditions. The observation that recruitment of EPO producing cells is reversed during prolonged continuous hypoxia seems compatible with both increases in tissue oxygenation as well as cellular adaptation to hypoxia.
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页码:815 / 823
页数:9
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