A, illustration of the typical labelling in a representative control cat (a) and three experimental animals submitted to unilateral vestibular neurectomy and observed 1 week (b), 3 weeks (c), and 3 months (d) after the lesion, and two representative cats subjected to a two- (e) or a one-step (f) bilateral vestibular neurectomy. Note that the lesion induced a strong increase in histidine decarboxylase mRNA expression in the tuberomammillary nuclei with predominance on the lesioned side at the 1- and 3-week survival times (b and c). Three months after UVN, HDC mRNA expression regained control levels on both sides (d). The two-step bilateral vestibular neurectomized cats (e), which are compensated left UVN cats killed 1 week after a second neurectomy on the right side, showed mirror images of what was observed after left UVN (b). Cats killed 1 week after a one-step bilateral vestibular lesion (f) showed HDC mRNA expression similar to that of control cats (a). F: fornix; TM: tuberomammillary nucleus; 3V: third ventricle. Bar, 1 mm. B, quantitative evaluation. Data are the mean values (±s.e.m.) of the labelled surface expressed in pixel2 for the control cats (N = 4), unilateral neurectomized cats (N = 12), and bilateral neurectomized cats (N = 8). The values recorded on the right (grey bars) and left (white bars) sides are given separately for all the subgroups of cats. The data from both sides were pooled for the controls (black bars) for a direct comparison with the subgroups of cats killed 1 week (b), 3 weeks (c) and 3 months (d) after a left unilateral vestibular neurectomy, and with the two-step (e) and the one-step (f) bilateral vestibular neurectomized cats. *P < 0. 01; **P < 0.0001; +P < 0.04. HDC: histidine decarboxylase; UVN: unilateral vestibular neurectomy; BVN: bilateral vestibular neurectomy; 1 W: 1 week; 3 W: 3 weeks; 3M: 3 months.