Rapid Detection of Donor Cell Free DNA in Lung Transplant Recipients with Rejections Using Donor-recipient HLA Mismatch

Overview

Journal Hum Immunol

Specialty Allergy & Immunology

Date 2017 Mar 8

PMID 28267558

Citations 23

Authors

Jun Zou

Brian Duffy

Michael Slade

Andrew Lee Young

Nancy Steward

Ramsey Hachem

T Mohanakumar

Affiliations

Soon will be listed here.

Abstract

Fiberoptic bronchoscopy and transbronchial lung biopsy are currently the gold standard for detection of acute rejection following human lung transplantation (LTx). However, these surveillance procedures are expensive and invasive. Up to now, there are few new methods that have demonstrated clinical utility for detecting early stages of rejection following human lung transplantation. We optimized and technically validated a novel method to quantify donor-derived circulating cell free DNA (DcfDNA) that can be used as an early biomarker for lung allograft rejection. The method involves the initial development of a panel of probes in which each probe will specifically target a unique sequence of a human leukocyte antigen (HLA) allele. After transplantation, donor/recipient specific probes are chosen based on the mismatched HLA loci, followed by droplet digital PCR (ddPCR) used as a quantitative assay to accurately track the trace amount of DcfDNA in an ample excess of recipient DNA background. The average false positive rate noted was about 1 per 800,000 molecules. Serially 2-fold diluted cfDNA, representing donor fractions of cfDNA, were spiked into a constant level of cfDNA representing the recipient cfDNA. The fraction of spiked cfDNA was measured and quantitative linearity was observed across seven serially diluted cfDNA samples. We were able to measure the minor portion of cfDNA as low as 0.2% of total cfDNA. We subsequently applied the method to a pilot set of 18 LTx recipients grouped into biopsy-proven acute rejection, bronchiolitis obliterans syndrome (BOS) or stable groups. Serial plasma samples were used to identify the percentage of DcfDNA over total cfDNA. The level of DcfDNA was significantly elevated in patients diagnosed with acute rejection (10.30±2.80, n=18), compared to that from stable (1.71±0.50, n=24) or from BOS patients (2.52±0.62, n=20). In conclusion, we present results validating the application of digital PCR to quantify DcfDNA assay in primary clinical specimens, which demonstrate that DcfDNA can be used as an early non-invasive biomarker for acute lung allograft rejection.

Citing Articles

Donor-derived Cell-free DNA Evaluation in Pediatric Heart Transplant Recipients: A Single-center 12-mo Experience.

Sorbini M, Aidala E, Carradori T, Vallone F, Togliatto G, Caorsi C Transplant Direct. 2024; 10(10):e1689.

PMID: 39301559 PMC: 11410329. DOI: 10.1097/TXD.0000000000001689.

Circulating donor-derived cell-free DNA as a marker for rejection after lung transplantation.

Li Y, Liang B Front Immunol. 2023; 14:1263389.

PMID: 37885888 PMC: 10598712. DOI: 10.3389/fimmu.2023.1263389.

Clinical relevance of cell-free DNA quantification and qualification during the first month after lung transplantation.

Pedini P, Coiffard B, Cherouat N, Casas S, Fina F, Boutonnet A Front Immunol. 2023; 14:1183949.

PMID: 37180126 PMC: 10174290. DOI: 10.3389/fimmu.2023.1183949.

Comparison of methods for donor-derived cell-free DNA quantification in plasma and urine from solid organ transplant recipients.

Kueng N, Arcioni S, Sandberg F, Kuhn C, Banz V, Largiader C Front Genet. 2023; 14:1089830.

PMID: 36777723 PMC: 9916053. DOI: 10.3389/fgene.2023.1089830.

Validation of a Simple, Rapid, and Cost-Effective Method for Acute Rejection Monitoring in Lung Transplant Recipients.

Sorbini M, Togliatto G, Mioli F, Simonato E, Marro M, Cappuccio M Transpl Int. 2022; 35:10546.

PMID: 35755857 PMC: 9221674. DOI: 10.3389/ti.2022.10546.

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