℮-conome: an automated tissue counting platform of cone photoreceptors for rodent models of retinitis pigmentosa

A Kastner; A Viczian; AC Fintz; AJ Jimenez; BM Bolstad; C Bowes; C Punzo; C Punzo; Emmanuelle Clérin; ET Camacho; F Chalmel; I Ivanovic; J Bennett; JC Blanks; JM Garcia-Fernandez; José-Alain Sahel; K Komeima; LD Carter-Dawson; MM LaVail; MN Delyfer; NB Haider; Nicolas Wicker; Olivier Poch; S Mohand-Said; S Reichman; Saddek Mohand-Saïd; T Cronin; T Cronin; T Leveillard; T Leveillard; Thierry Léveillard; UT Byrne; Y Yang

℮-conome: an automated tissue counting platform of cone photoreceptors for rodent models of retinitis pigmentosa

Authors: A Kastner
A Viczian
AC Fintz
AJ Jimenez
BM Bolstad
C Bowes
C Punzo
C Punzo
Emmanuelle Clérin
ET Camacho
F Chalmel
I Ivanovic
J Bennett
JC Blanks
JM Garcia-Fernandez
José-Alain Sahel
K Komeima
LD Carter-Dawson
MM LaVail
MN Delyfer
NB Haider
Nicolas Wicker
Olivier Poch
S Mohand-Said
S Reichman
Saddek Mohand-Saïd
T Cronin
T Cronin
T Leveillard
T Leveillard
Thierry Léveillard
UT Byrne
Y Yang
Publication date: 1 January 2011
Publisher: BioMed Central
Doi

Abstract

Abstract Background Retinitis pigmentosa is characterized by the sequential loss of rod and cone photoreceptors. The preservation of cones would prevent blindness due to their essential role in human vision. Rod-derived Cone Viability Factor is a thioredoxin-like protein that is secreted by rods and is involved in cone survival. To validate the activity of Rod-derived Cone Viability Factors (RdCVFs) as therapeutic agents for treating retinitis Pigmentosa, we have developed e-conome, an automated cell counting platform for retinal flat mounts of rodent models of cone degeneration. This automated quantification method allows for faster data analysis thereby accelerating translational research. Methods An inverted fluorescent microscope, motorized and coupled to a CCD camera records images of cones labeled with fluorescent peanut agglutinin lectin on flat-mounted retinas. In an average of 300 fields per retina, nine Z-planes at magnification X40 are acquired after two-stage autofocus individually for each field. The projection of the stack of 9 images is subject to a threshold, filtered to exclude aberrant images based on preset variables. The cones are identified by treating the resulting image using 13 variables empirically determined. The cone density is calculated over the 300 fields. Results The method was validated by comparison to the conventional stereological counting. The decrease in cone density in <it>rd1 </it>mouse was found to be equivalent to the decrease determined by stereological counting. We also studied the spatiotemporal pattern of the degeneration of cones in the <it>rd1 </it>mouse and show that while the reduction in cone density starts in the central part of the retina, cone degeneration progresses at the same speed over the whole retinal surface. We finally show that for mice with an inactivation of the Nucleoredoxin-like genes <it>Nxnl1 </it>or <it>Nxnl2 </it>encoding RdCVFs, the loss of cones is more pronounced in the ventral retina. Conclusion The automated platform ℮-conome used here for retinal disease is a tool that can broadly accelerate translational research for neurodegenerative diseases.</p