4.2 Article

The impact of Nucleofection® on the activation state of primary human CD4 T cells

期刊

JOURNAL OF IMMUNOLOGICAL METHODS
卷 408, 期 -, 页码 123-131

出版社

ELSEVIER SCIENCE BV
DOI: 10.1016/j.jim.2014.05.014

关键词

Nucleofection (R); Gene transfer; T cell activation; Calcium; HIV-1; Plasmid

资金

  1. NIH [R01-AR-48257, R21-AR-49335, R21-AI-68574]

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Gene transfer into primary human CD4 T lymphocytes is a critical tool in studying the mechanism of T cell-dependent immune responses and human immunodeficiency virus-1 (HIV-1) infection. Nucleofection (R) is an electroporation technique that allows efficient gene transfer into primary human CD4 T cells that are notoriously resistant to traditional electroporation. Despite its popularity in immunological research, careful characterization of its impact on the physiology of CD4 T cells has not been documented. Herein, using freshly-isolated primary human CD4 T cells, we examine the effects of Nucleofection (R) on CD4 T cell morphology, intracellular calcium levels, cell surface activation markers, and transcriptional activity. We find that immediately after Nucleofection (R), CD4 T cells undergo dramatic morphological changes characterized by wrinkled and dilated plasma membranes before recovering 1 h later. The intracellular calcium level also increases after Nucleofection (R), peaking after 1 h before recovering 8 h post transfection. Moreover, Nucleofection (R) leads to increased expression of T cell activation markers, CD154 and CD69, for more than 24 h, and enhances the activation effects of phytohemagglutinin (PHA) stimulation. In addition, transcriptional activity is increased in the first 24 h after Nucleofection (R), even in the absence of exogenous stimuli. Therefore, Nucleofection (R) significantly alters the activation state of primary human CD4 T cells. The effect of transferred gene products on CD4 T cell function by Nucleofection (R) should be assessed after sufficient resting time post transfection or analyzed in light of the activation caveats mentioned above. (C) 2014 Elsevier B.V. All rights reserved.

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