Infant luminance and chromatic contrast sensitivity: optokinetic nystagmus data on 3-month-olds.

Infant color vision is poor, and most psychophysical experiments agree that infant color vision emerges between ages 3 weeks and 3 months. Presumably, the color vision of infants is poor during the months immediately after it has emerged. We have tested two alternative explanations for the poor color vision of infants: (1) there is a special critical immaturity within the color pathways of infants; (2) infants have poor infant color vision because they are insensitive to contrast. Luminance and chromatic contrast thresholds were measured on 3-month-olds using optokinetic nystagmus (OKN), and adult luminance and chromatic contrast thresholds were measured using OKN and two forced-choice methods: direction-of-motion discrimination and grating detection. The infant chromatic-to-luminance contrast threshold ratio shows that infants are as sensitive or even more sensitive than adults to color, depending on the testing method used on adults. This result suggests that the general contrast insensitivity hypothesis is correct. Conservative "worst-case" quantitative analysis strongly suggests that this result is not the consequence of a luminance artifact.

Hyperplastic G cell responsiveness in vitro.

To evaluate the responsiveness of isolated, hyperplastic antral gastrin-producing G cells to a variety of secretagogues, hyperplastic hypergastrinemia was produced in Sprague-Dawley rats by fundusectomy. Mean serum immunoreactive gastrin (IRG) concentration was elevated fivefold above controls 4 days after operation and rose steadily to an eightfold increase at 66 days. Mean antral G cell density remained at control levels for as long as 7 days, increased twofold at 14 days, then remained between twofold and threefold greater than controls for as long as 66 days after operation. Antral mucosa IRG content increased from 141 +/- 38 (control) to 262 +/- 58 ng IRG/gm mucosa (4 to 6 weeks after fundusectomy). Crude fractions of dispersed antral mucosa cells enriched in G cells from fundusectomized rats contained 6.5% +/- 1.4% G cells with 0.19 +/- 0.6 pg IRG/G cell. Corresponding preparations from nonoperated rats contained 5.1% +/- 0.5% G cells with 0.07 +/- 0.02 pg IRG/G cell. Viability averaged greater than 95% for all preparations. Gastrin secretion was monitored in cell preparations further enriched in G cells (9% to 10%) by Percoll density gradient centrifugation either in the absence (basal) or presence of bombesin (1 mumol, 1 nmol/L), carbachol (1 mmol/L), leucine (10 mmol/L), and ethylamine (10 mmol/L). The basal secretory rate of hyperplastic G cell populations averaged 250% greater than normal G cell basal rates. Hyperplastic G cell preparations had an increased IRG secretory rate in the presence of bombesin (1 mumol/L, 750%; 1 nmol/L, 191%), leucine (120%), ethylamine (236%), and carbachol (183%). These conditions failed to increase the IRG secretory rate above basal in preparations from normal antra. Viable, dispersed, hyperplastic G cells have increased IRG content and basal IRG secretory rate and are functionally responsive to a variety of secretagogues.

Identification of gastrin-producing cells in cell cultures and smears: an avidin-biotin-peroxidase complex (ABC) technique.

A method is described that uses the avidin-biotin complex (ABC) immunoperoxidase technique to provide a rapid, sensitive, and specific means to quantitate isolated G cells in cultures and suspensions.