| Literature DB >> 14604536 |
Shiro Kanegasaki1, Yuka Nomura, Nao Nitta, Shuichi Akiyama, Takuya Tamatani, Yasuhiro Goshoh, Takashi Yoshida, Tsuyoshi Sato, Yuji Kikuchi.
Abstract
We have developed an optically accessible, horizontal chemotaxis apparatus consisting of an etched silicon substrate and a flat glass plate, both of which form two compartments with a 5-microm-deep microchannel in between. The device is held together with a stainless steel holder with holes for injecting cells and a chemoattractant to the different compartments. Migration of cells in the channel is traced with time-lapse intervals using a CCD camera. By developing a method for aligning cells at the edge of the channel, we could successfully reduce the number of cells required for a chemotactic assay, depending on the experiment, to 100 or less. To prevent ceaseless flow of contents between the adjacent compartments via the communicating microchannel, a space at the top end of the holder was filled with medium after aligning the cells. By using a fluorescent probe, we demonstrated experimentally that a stable concentration gradient could be maintained. Furthermore, we determined theoretical details of the gradient established using a model chemokine and a computational fluid dynamics code. Reproducible kinetic results of cell migration were obtained using human neutrophils and IL-8 as a model. Migration of other cells such as eosinophils, basophils and Jurkat lymphocytes toward the appropriate chemokines were also demonstrated.Entities:
Mesh:
Year: 2003 PMID: 14604536 DOI: 10.1016/j.jim.2003.07.008
Source DB: PubMed Journal: J Immunol Methods ISSN: 0022-1759 Impact factor: 2.303