Our goal is to speed standardization of sample sparing assays of immune function through the design and validation of a flexible microfluidic system that is capable of automated processing and multi-parameter analysis of rare cells. A novel cell capture mechanism (Vortex cell trapping) is utilized to isolate rare cells into nanolier arrays, and fully automate the steps involved in profiling cell function (i.e., activation, incubaton, labeling). We utilize the device to perform sample sparing versions of two important assays of immune function: the CD154 and peptide-MHC tetramer assay, and investigate the effect of common processing steps on the detection limits and variability at input sample volumes that are beyond the limits of existing methods. Unlike current microfluidic systems, our approach enables direct capture of cells from complex clinical samples, isolation and monitoring of antigen-specific cells, and rapid exchange of buffer around the cells for processing without loss. In addition, the microfluidic traps are designed for direct, post-process ejection of the cells to existing multi-parameter analytical platforms (i.e., cell surface marker, transcription level, or TCR sequence analysis) to enable faster translation to clinical labs. The Vortex trap allows direct ex vivo cytokine secretion profiling of rare cells through peptide-MHC tetramer or CD154-based capture. Both of these assays have recently enabled direct monitoring of functional immune response in large-volume clinical samples. However, analysis of antigen-specific cells in volume or cell limited biological specimens remains challenging, and an automated method for ex vivo secretion profiling is desired. As such, we propose to analytically validate our cytokine profiling assay using both a multiple sclerosis (MS) (e.g., clinical need to analyze rare cells with pathogenic secretion profiles), and viral vaccine model (e.g., clinical need to screen functional response of cells from low sample volumes). Clinical validation will be performed using patient-derived samples, and will include direct comparisons to the current standard assays (i.e., T cell cloning or flow-cytometer-based pMHC tetramer or CD154 assays). Our approach is supported by strong preliminary data, and we have assembled a strong academic-industrial partnership consisting of UCLA (Vortex cell trapping), Yale University/Benaroya Research Institute (pMHC tetramers, T cell lines, and patient samples), and GE Global Research (cell-cytokine capture beads, and analytical interface).

Public Health Relevance

The goal of this proposal is to perform sample sparing assays of immune cell function from minute samples volumes. We accomplish this through the use of a novel microfluidic device that enables the capture and cytokine secretion profiling of rare immune cells, from as little as 25 microliters of blood. We propose to clinically validate this unique device and assay using both multiple sclerosis (rare auto-reactive cells) and vaccinated (abundant viral-reactive cells) patient samples.

Agency
National Institute of Health (NIH)
Institute
National Institute of Allergy and Infectious Diseases (NIAID)
Type
Resource-Related Research Projects--Cooperative Agreements (U24)
Project #
5U24AI118667-03
Application #
9279045
Study Section
Special Emphasis Panel (ZAI1-MM-I (M1))
Program Officer
Bourcier, Katarzyna
Project Start
2015-06-26
Project End
2020-05-31
Budget Start
2017-06-01
Budget End
2018-05-31
Support Year
3
Fiscal Year
2017
Total Cost
$377,389
Indirect Cost
$104,223
Name
General Electric Global Research Center
Department
Type
Research Institutes
DUNS #
086188401
City
Niskayuna
State
NY
Country
United States
Zip Code
12309
Murray, Coleman; Pao, Edward; Jann, Andrew et al. (2018) Continuous and Quantitative Purification of T-Cell Subsets for Cell Therapy Manufacturing Using Magnetic Ratcheting Cytometry. SLAS Technol 23:326-337
Murray, Coleman; Miwa, Hiromi; Dhar, Manjima et al. (2018) Unsupervised capture and profiling of rare immune cells using multi-directional magnetic ratcheting. Lab Chip 18:2396-2409