Urinary mRNA for the Diagnosis of Renal Allograft Rejection: The Issue of Normalization

被引:14
|
作者
Galichon, P. [1 ,2 ,3 ]
Amrouche, L. [4 ]
Hertig, A. [1 ,2 ,3 ]
Brocheriou, I. [1 ,2 ,5 ]
Rabant, M. [6 ]
Xu-Dubois, Y. -C. [1 ]
Ouali, N. [3 ]
Dahan, K. [7 ]
Morin, L. [8 ]
Terzi, F. [4 ]
Rondeau, E. [1 ,2 ,3 ]
Anglicheau, D. [4 ,8 ,9 ,10 ]
机构
[1] Hop Tenon, INSERM, U1155, Paris, France
[2] Sorbonne Univ, Univ Paris 06, Paris, France
[3] Hop Tenon, AP HP, Urgences Nephrol & Transplantat Renale, Paris, France
[4] Hop Necker Enfants Malad, INSERM, U1151, Paris, France
[5] Hop Tenon, AP HP, Serv Anat Pathol, Paris, France
[6] Hop Necker Enfants Malad, AP HP, Anat Pathol Lab, Paris, France
[7] Hop Necker Enfants Malad, AP HP, Serv Nephrol & Dialyses, Paris, France
[8] Hop Necker Enfants Malad, AP HP, Serv Nephrol & Transplantat Adulte, Paris, France
[9] Univ Paris 05, Sorbonne Paris Cite, Paris, France
[10] Hop Necker Enfants Malad, RTRS Centaure Labex Transplantex, Paris, France
关键词
OPTIMIZATION; VIRUS; TIME;
D O I
10.1111/ajt.13891
中图分类号
R61 [外科手术学];
学科分类号
摘要
Urinary messenger RNA (mRNA) quantification is a promising method for noninvasive diagnosis of renal allograft rejection (AR), but the quantification of mRNAs in urine remains challenging due to degradation. RNA normalization may be warranted to overcome these issues, but the strategies of gene normalization have been poorly evaluated. Herein, we address this issue in a case-control study of 108 urine samples collected at time of allograft biopsy in kidney recipients with (n = 52) or without (n = 56) AR by comparing the diagnostic value of IP-10 and CD3 epsilon mRNAs-two biomarkers of AR-after normalization by the total amount of RNA, normalization by one of the three widely used reference RNAs-18S, glyceraldehyde-3-phosphate dehydrogenase (GAPDH) and Hypoxanthine-guanine phosphoribosyltransferase (HPRT)or normalization using uroplakin 1A (UPK) mRNA as a possible urine-specific reference mRNA. Our results show that normalization based on the total quantity of RNA is not substantially improved by additional normalization and may even be worsened with some classical reference genes that are overexpressed during rejection. However, considering that normalization by a reference gene is necessary to ensure polymerase chain reaction (PCR) quality and reproducibility and to suppress the effect of RNA degradation, we suggest that GAPDH and UPK1A are preferable to 18S or HPRT RNA.
引用
收藏
页码:3033 / 3040
页数:8
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