Humanized mouse models reveal an immunologic classification of idiopathic CD4 lymphocytopenia subtypes
Ainhoa Perez-Diez, … , David F. Stroncek, Irini Sereti
Ainhoa Perez-Diez, … , David F. Stroncek, Irini Sereti
Published July 25, 2019
Citation Information: JCI Insight. 2019;4(14):e127802. https://doi.org/10.1172/jci.insight.127802.
View: Text | PDF
Research Article Immunology Infectious disease

Humanized mouse models reveal an immunologic classification of idiopathic CD4 lymphocytopenia subtypes

Abstract

Idiopathic CD4 lymphocytopenia (ICL) is a clinically heterogeneous immunodeficiency disorder defined by low numbers of circulating CD4+ T cells and increased susceptibility to opportunistic infections. CD8+ T cells, NK, and/or B cells may also be deficient in some patients. To delineate possible pathogenic cellular mechanisms in ICL, we compared immune system development and function in NOD-RAGKO-γcKO (NRG) mice transplanted with hematopoietic stem cells from patients with ICL or healthy controls. CD34+ hematopoietic stem cells from healthy controls and patients with ICL reconstituted NRG mice equally well. In contrast, PBMC transfers into NRG mice identified 2 ICL engraftment phenotypes, reconstituting and nonreconstituting (NR), based on the absence or presence of donor lymphopenia. For patients in the NR group, the distribution of lymphocyte subsets was similar in the peripheral blood of both the patient and the corresponding humanized mice. The NR-ICL group could be further divided into individuals whose CD3+ T cells had defects in proliferation or survival. Thus, ICL cellular pathogenesis might be classified by humanized mouse models into 3 distinct subtypes: (a) T cell extrinsic, (b) T cell intrinsic affecting proliferation, and (c) T cell intrinsic affecting survival. Humanized mouse models of ICL help to delineate etiology and ultimately to guide development of individualized therapeutic strategies.

Authors

Ainhoa Perez-Diez, Xiangdong Liu, Virginia Sheikh, Gregg Roby, David F. Stroncek, Irini Sereti

×

Figure 4

ICL is phenocopied in NRG mice receiving ICL PBMCs.

Options: View larger image (or click on image) Download as PowerPoint
ICL is phenocopied in NRG mice receiving ICL PBMCs. (A) Percentage of CD...
(A) Percentage of CD3+, CD4+, CD8+, and TCR-γδ+ T cells in blood of hPBMC mice at days 3, 14, and 28 after transfer of PBMCs from HC (black) or patients ICL-26 (blue) or ICL-45 (pink). All percentages calculated from the live lymphocyte gate. Insert represents the number of CD4+, CD8+, and CD3+CD4CD8 cells (where γδT cells are included) that each experimental group of mice received. (B) Representative dot plots (left) and compiled data (right), showing the percentage of hCD45+CD3+ cells found in spleen, LN, bone marrow, and liver, 4 weeks after PBMC transfer, gated on live events. (C) Numbers of CD4+, CD8+, γδT cells, and B cells found in spleens of hPBMC mice 4 weeks after PBMC transfer. (D) Percentages of the different populations found within the live hCD45+ gate in either the original PBMC inoculum (left) or in the spleen of individual mice 4 weeks after PBMC transfer (right). When the total percentage does not add up to 100, it is due to a subset of events that were hCD45+ but negative for any of the markers used. (AD) Data from the same experiment; the same symbols represent the same individual mice.