The adhesion of mouse embryonic brain cells was measured in a rotating chamber. A method is proposed for quantitative evaluation of adhesion kinetics. Dissociated cells were incubated in a planparallel chamber and pictures were taken between time 0-120 min. Film negatives were evaluated by computer--controlled scanning. Ten thousand individual data area obtained from one frame and 1,000 levels of absorbency are distinguished. A method is described which allows the discrimination of area, density and the shape of adhering cells. The influence of the dissociation procedure on cellular adhesion was studied. Short trypsinisation (0.025% trypsin for 5 min) followed by sieving was most favourable for adhesion. Mechanical sieving and dissociation with EGTA (Ca2+ chelator) gave less satisfactory results. Significantly diminished adhesion was observed after prolonged trypsinisation. If cells were incubated in media lacking Ca2+, adhesion was significantly inhibited. The kinetics of adhesion follows the curve of flocculation kinetics independently of the dissociation procedure and composition of the medium.

Ontogenetic analysis of some surface markers on pig lymphocytes using fluorescence-activated cell sorter