Measurement of corneal sublayer thickness and transparency in transgenic mice with altered corneal clarity using in vivo confocal microscopy

James V. Jester; Young Ghee Lee; Jie Li; Shukti Chakravarti; Jennifer Paul; Walter M Petroll; Harrison D Cavanagh

doi:10.1016/S0042-6989(00)00222-4

Measurement of corneal sublayer thickness and transparency in transgenic mice with altered corneal clarity using in vivo confocal microscopy

James V. Jester, Young Ghee Lee, Jie Li, Shukti Chakravarti, Jennifer Paul, Walter M Petroll, Harrison D Cavanagh

Research output: Contribution to journal › Article › peer-review

38 Scopus citations

Abstract

Measurement of sublayer thickness and transparency at cellular level in the living animal are critical to understanding the role of specific transgenes and transgene products in controlling corneal development and maintenance of transparency. Using two different transgenic mouse strains having altered corneal clarity, we have evaluated the ability of in vivo confocal microscopy to measure corneal haze and localize light scattering structures. Projection of 2-D and 3-D image information identified the nature and location of light scattering within the cornea and allowed correlation of unique structural differences to transgene expression. Our findings suggest that in vivo confocal microscopy can be used to identify the effects of transgene expression on mouse corneal transparency.

Original language	English (US)
Pages (from-to)	1283-1290
Number of pages	8
Journal	Vision Research
Volume	41
Issue number	10-11
DOIs	https://doi.org/10.1016/S0042-6989(00)00222-4
State	Published - 2001

Keywords

Confocal microscopy
Cornea
Digital imaging
Transgenic
Transparency

ASJC Scopus subject areas

Ophthalmology
Sensory Systems

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10.1016/S0042-6989(00)00222-4

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title = "Measurement of corneal sublayer thickness and transparency in transgenic mice with altered corneal clarity using in vivo confocal microscopy",

abstract = "Measurement of sublayer thickness and transparency at cellular level in the living animal are critical to understanding the role of specific transgenes and transgene products in controlling corneal development and maintenance of transparency. Using two different transgenic mouse strains having altered corneal clarity, we have evaluated the ability of in vivo confocal microscopy to measure corneal haze and localize light scattering structures. Projection of 2-D and 3-D image information identified the nature and location of light scattering within the cornea and allowed correlation of unique structural differences to transgene expression. Our findings suggest that in vivo confocal microscopy can be used to identify the effects of transgene expression on mouse corneal transparency.",

keywords = "Confocal microscopy, Cornea, Digital imaging, Transgenic, Transparency",

author = "Jester, {James V.} and {Ghee Lee}, Young and Jie Li and Shukti Chakravarti and Jennifer Paul and Petroll, {Walter M} and Cavanagh, {Harrison D}",

note = "Funding Information: This work was supported, in part, by grants EY07348 (JVJ), EY11654 (SC) and EY13215 (JVJ) from the National Eye Institute, Bethesda, MD, and Research to Prevent Blindness, Inc., New York, NY. ",

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doi = "10.1016/S0042-6989(00)00222-4",

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AU - Jester, James V.

AU - Ghee Lee, Young

AU - Li, Jie

AU - Chakravarti, Shukti

AU - Paul, Jennifer

AU - Petroll, Walter M

AU - Cavanagh, Harrison D

N1 - Funding Information: This work was supported, in part, by grants EY07348 (JVJ), EY11654 (SC) and EY13215 (JVJ) from the National Eye Institute, Bethesda, MD, and Research to Prevent Blindness, Inc., New York, NY.

PY - 2001

Y1 - 2001

N2 - Measurement of sublayer thickness and transparency at cellular level in the living animal are critical to understanding the role of specific transgenes and transgene products in controlling corneal development and maintenance of transparency. Using two different transgenic mouse strains having altered corneal clarity, we have evaluated the ability of in vivo confocal microscopy to measure corneal haze and localize light scattering structures. Projection of 2-D and 3-D image information identified the nature and location of light scattering within the cornea and allowed correlation of unique structural differences to transgene expression. Our findings suggest that in vivo confocal microscopy can be used to identify the effects of transgene expression on mouse corneal transparency.

AB - Measurement of sublayer thickness and transparency at cellular level in the living animal are critical to understanding the role of specific transgenes and transgene products in controlling corneal development and maintenance of transparency. Using two different transgenic mouse strains having altered corneal clarity, we have evaluated the ability of in vivo confocal microscopy to measure corneal haze and localize light scattering structures. Projection of 2-D and 3-D image information identified the nature and location of light scattering within the cornea and allowed correlation of unique structural differences to transgene expression. Our findings suggest that in vivo confocal microscopy can be used to identify the effects of transgene expression on mouse corneal transparency.

KW - Confocal microscopy

KW - Cornea

KW - Digital imaging

KW - Transgenic

KW - Transparency

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Measurement of corneal sublayer thickness and transparency in transgenic mice with altered corneal clarity using in vivo confocal microscopy

Abstract

Keywords

ASJC Scopus subject areas

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