A role for heterologous gap junctions between melanoma and endothelial cells in metastasis
Akihiko Ito, … , Hiroshi Yamasaki, Hiroshi Nojima
Akihiko Ito, … , Hiroshi Yamasaki, Hiroshi Nojima
Published May 1, 2000
Citation Information: J Clin Invest. 2000;105(9):1189-1197. https://doi.org/10.1172/JCI8257.
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A role for heterologous gap junctions between melanoma and endothelial cells in metastasis

Abstract

F10 and BL6 sublines of B16 mouse melanoma cells are metastatic after intravenous injection, but only BL6 cells are metastatic after subcutaneous injection. We found that connexin (Cx) 26 is upregulated in BL6 cells. To examine gap junction formation, we devised a coculture system, in which an opened vein segment was placed at the bottom of a culture dish and then dye-labeled melanoma cells were seeded onto it. Immunohistochemistry indicated that the vein segment preserved the integrity of the endothelial monolayer. In this system, BL6 cells could transfer dye into endothelial cells but F10 cells could not. Transfection with wild-type Cx26 rendered F10 cells competent for coupling with endothelial cells and as spontaneously metastatic as BL6 cells. Conversely, transfection with a dominant-negative form of Cx26 rendered BL6 cells deficient in coupling and less metastatic. In human melanoma lesions, the level of Cx26 expression was low in melanoma cells residing in the basal layer, but significantly upregulated in melanoma cells invading the dermis. The results suggested that Cx26 plays a role in intravasation and extravasation of tumor cells through heterologous gap junction formation with endothelial cells.

Authors

Akihiko Ito, Fumitaka Katoh, Tatsuki R. Kataoka, Morihito Okada, Noriaki Tsubota, Hideo Asada, Kunihiko Yoshikawa, Sakan Maeda, Yukihiko Kitamura, Hiroshi Yamasaki, Hiroshi Nojima

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Figure 4

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Spontaneous metastasis assay of Cx26 and Cx32 transfectants. (a) Primary...
Spontaneous metastasis assay of Cx26 and Cx32 transfectants. (a) Primary tumor growth at the inoculation site (right footpad). Growth curves for the five representative clones are expressed as the mean and SE of three independent experiments. The values of the other clones used were within the range of these five clones at any time point. There was no significant difference between the clones. (b) The number of colonies in the lungs produced by various F10 and BL6 clones. F10-pcDNA3 and BL6-pcDNA3 clones are vector controls. Data are expressed as the mean and SE of three independent experiments. AP < 0.05 by t test when compared with the value obtained from F10 cells. BP < 0.05 by t test when compared with the value obtained from BL6 cells. The Northern blot shows the detection of endogenous and exogenous Cx26 and Cx32 mRNA in each clone. (c) Representative results of the lung metastatic colonies produced by F10, BL6, F10-Cx26WT-1, and BL6-Cx26C60F-1 cells. Note that BL6 and BL6-Cx26C60F-1 cells produced solid black colonies whereas F10-Cx26WT-1 cells produced amelanotic colonies as well as melanotic ones.