Universal monitoring of minimal residual disease in acute myeloid leukemia
Elaine Coustan-Smith, … , James R. Downing, Dario Campana
Elaine Coustan-Smith, … , James R. Downing, Dario Campana
Published May 3, 2018
Citation Information: JCI Insight. 2018;3(9):e98561. https://doi.org/10.1172/jci.insight.98561.
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Clinical Research and Public Health Hematology Oncology

Universal monitoring of minimal residual disease in acute myeloid leukemia

Abstract

BACKGROUND. Optimal management of acute myeloid leukemia (AML) requires monitoring of treatment response, but minimal residual disease (MRD) may escape detection. We sought to identify distinctive features of AML cells for universal MRD monitoring. METHODS. We compared genome-wide gene expression of AML cells from 157 patients with that of normal myeloblasts. Markers encoded by aberrantly expressed genes, including some previously associated with leukemia stem cells, were studied by flow cytometry in 240 patients with AML and in nonleukemic myeloblasts from 63 bone marrow samples. RESULTS. Twenty-two (CD9, CD18, CD25, CD32, CD44, CD47, CD52, CD54, CD59, CD64, CD68, CD86, CD93, CD96, CD97, CD99, CD123, CD200, CD300a/c, CD366, CD371, and CX3CR1) markers were aberrantly expressed in AML. Leukemia-associated profiles defined by these markers extended to immature CD34+CD38– AML cells; expression remained stable during treatment. The markers yielded MRD measurements matching those of standard methods in 208 samples from 52 patients undergoing chemotherapy and revealed otherwise undetectable MRD. They allowed MRD monitoring in 129 consecutive patients, yielding prognostically significant results. Using a machine-learning algorithm to reduce high-dimensional data sets to 2-dimensional data, the markers allowed a clear visualization of MRD and could detect 1 leukemic cell among more than 100,000 normal cells. CONCLUSION. The markers uncovered in this study allow universal and sensitive monitoring of MRD in AML. In combination with contemporary analytical tools, the markers improve the discrimination between leukemic and normal cells, thus facilitating data interpretation and, hence, the reliability of MRD results. FUNDING. National Cancer Institute (CA60419 and CA21765); American Lebanese Syrian Associated Charities; National Medical Research Council of Singapore (1299/2011); Viva Foundation for Children with Cancer, Children’s Cancer Foundation, Tote Board & Turf Club, and Lee Foundation of Singapore.

Authors

Elaine Coustan-Smith, Guangchun Song, Sheila Shurtleff, Allen Eng-Juh Yeoh, Wee Joo Chng, Siew Peng Chen, Jeffrey E. Rubnitz, Ching-Hon Pui, James R. Downing, Dario Campana

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Figure 7

Improved discrimination of AML and normal cells with the additional markers.

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Improved discrimination of AML and normal cells with the additional mark...
(A) tSNE analysis of the cell profile of normal bone marrow CD34, CD117, CD45, and CD33 mononucleated cells from 4 donors (shown in blue) mixed with various proportions of AML cells (shown in red). The percentage of AML cells in each mixture is shown. (B) MRD visualization in bone marrow mononucleated cells from a patient with AML after the first cycle of remission induction chemotherapy. Cells were labeled with either the best available standard markers (CD38, CD133, CD7, and anti-HLA-Dr) or with CD52 and CD47; both sample aliquots were also labeled with CD34, CD117, CD45, and CD33. tSNE was performed on gated myeloid CD34+ cells. The percentage estimated MRD (red contour plots) according to CD52 and CD47 is shown. (C) MRD visualization in bone marrow mononucleated cells from another patient with AML after the second cycle of remission induction chemotherapy. Cells were labeled with CD34, CD117, CD45, and CD33, in combination with CD7 (the best standard marker in this case) and CD96 (see Supplemental Figure 1B for details on the analysis process). The percentage estimated MRD (red contour plots) according to CD7 plus CD96 is shown; histograms illustrate the individual marker expression in normal (blue) versus AML cells (red). (D) tSNE analysis of the cell profile of normal bone marrow CD34+CD33+CD117+ mononucleated cells from 10 donors (blue) containing various proportions of AML cells (red). The histograms on the right show expression of the individual markers on the leukemia cell cluster (red) compared with the remaining cells (blue).