12415310

pubmed:Citation

11

Many lymphocyte functions, such as antigen recognition, take place deep in densely populated lymphoid organs. Because direct in vivo observation was not possible, the dynamics of immune-cell interactions have been inferred or extrapolated from in vitro studies. Two-photon fluorescence excitation uses extremely brief (<1 picosecond) and intense pulses of light to 'see' directly into living tissues, to a greater depth and with less phototoxicity than conventional imaging methods. Two-photon microscopy, in combination with newly developed indicator molecules, promises to extend single-cell approaches to the in vivo setting and to reveal in detail the cellular collaborations that underlie the immune response.

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http://linkedlifedata.com/resource/pubmed/journal/101124169

MEDLINE

1474-1733

Print

NLM

872-80

pubmed-meshheading:12415310-Animals, pubmed-meshheading:12415310-Diagnostic Imaging, pubmed-meshheading:12415310-Humans, pubmed-meshheading:12415310-Microscopy, Confocal, pubmed-meshheading:12415310-Photons, pubmed-meshheading:12415310-T-Lymphocytes

Two-photon tissue imaging: seeing the immune system in a fresh light.

Journal Article, Research Support, U.S. Gov't, P.H.S., Review