Abstract

Confocal microscopes provide superior optical sectioning, without the effect of out-of-focus light that usually compromises the quality and usefulness of light images, especially those using fluorescent probes. A series of confocal images at increasing depths in the specimen is processed for 3D reconstruction of objects labeled with fluorescent dyes or visualized by reflection, using software provided by the manufacturer plus software written in this facility. Our Leica confocal microscope incorporates an upright microscope, and has an argon-krypton laser for improved double and triple fluorescent labeling. It has two reflected/epifluorescent light detectors, and on transmitted light, non-confocal detector. Images are stored on disk during the working day, and either transferred to the users own computer or one of our image-analysis workstations using FTP, or written to optical disk for archival storage, so that the hard disk can be cleared for other users. Users are introduced to the instrument, and usually for one or two sessions, the operation is done entirely by laboratory personnel, unless of course the user already has confocal experience. Subsequently, users operate the instrument under supervision, and eventually can work alone. Sets of rules help to protect the instrument from incorrect or careless use. The instrument is housed in the resource and thus always is under the control and supervision of resource personnel. During the current grant year, we have had a total of 13 different laboratories making significant use of the confocal microscope. This represented approximately 22 different projects, and 4 institutions. Usage is very high, with the instrument in use during the day, at night, and often on weekends. We are seeking to obtain an additional instrument to relieve this heavy load. We had to replace our argon/krypton laser during the current year as the original tube failed. We also replaced the PC computer that forms the operator interface, because of intermittent software failures that we could not track down, but that disappeared when we made a temporary substitution of the entire computer. A new computer was purchased. 8-31-96

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Center for Research Resources (NCRR)
Type
Biotechnology Resource Grants (P41)
Project #
5P41RR002483-10
Application #
5224051
Study Section
Project Start
Project End
Budget Start
Budget End
Support Year
10
Fiscal Year
1996
Total Cost
Indirect Cost

  Publications

Deng, Manqi; Williams, Carmen J; Schultz, Richard M (2005) Role of MAP kinase and myosin light chain kinase in chromosome-induced development of mouse egg polarity. Dev Biol 278:358-66
Tutuncu, Levent; Stein, Paula; Ord, Teri S et al. (2004) Calreticulin on the mouse egg surface mediates transmembrane signaling linked to cell cycle resumption. Dev Biol 270:246-60
Brown, Rebecca L; August, Shelley L; Williams, Carmen J et al. (2003) AKAP7gamma is a nuclear RI-binding AKAP. Biochem Biophys Res Commun 306:394-401
Deng, Manqi; Kishikawa, Hidefumi; Yanagimachi, Ryuzo et al. (2003) Chromatin-mediated cortical granule redistribution is responsible for the formation of the cortical granule-free domain in mouse eggs. Dev Biol 257:166-76
Brown, Rebecca L; Ord, Teri; Moss, Stuart B et al. (2002) A-kinase anchor proteins as potential regulators of protein kinase A function in oocytes. Biol Reprod 67:981-7
Li, J; Zhu, X; Ashton, F T et al. (2001) Sensory neuroanatomy of a passively ingested nematode parasite, Haemonchus contortus: amphidial neurons of the third-stage larva. J Parasitol 87:65-72
Robson, P; Stein, P; Zhou, B et al. (2001) Inner cell mass-specific expression of a cell adhesion molecule (PECAM-1/CD31) in the mouse blastocyst. Dev Biol 234:317-29
Travis, A J; Merdiushev, T; Vargas, L A et al. (2001) Expression and localization of caveolin-1, and the presence of membrane rafts, in mouse and Guinea pig spermatozoa. Dev Biol 240:599-610
Stein, P; Schultz, R M (2000) Initiation of a chromatin-based transcriptionally repressive state in the preimplantation mouse embryo: lack of a primary role for expression of somatic histone H1. Mol Reprod Dev 55:241-8
Li, J; Ashton, F T; Gamble, H R et al. (2000) Sensory neuroanatomy of a passively ingested nematode parasite, Haemonchus contortus: amphidial neurons of the first stage larva. J Comp Neurol 417:299-314

Showing the most recent 10 out of 38 publications