MMP and TIMP expression in quiescent, dividing, and differentiating human lens cells

Lisa M. Hodgkinson; George Duncan; Lixin Wang; Caroline J. Pennington; Dylan R. Edwards; I. Michael Wormstone

doi:10.1167/iovs.06-1371

MMP and TIMP expression in quiescent, dividing, and differentiating human lens cells

Lisa M. Hodgkinson, George Duncan, Lixin Wang, Caroline J. Pennington, Dylan R. Edwards, I. Michael Wormstone

Research output: Journal Publication › Article › peer-review

21 Citations (Scopus)

Abstract

PURPOSE. Matrix metalloproteinases (MMPs) and the tissue inhibitors of the MMPs (TIMPs) have been implicated in lens differentiation, growth, remodeling, and cataract. Hence, a gene expression analysis was undertaken in epithelial and fiber cells dissected from clear human donor lenses. METHODS. The human lens was dissected into three regions: anterior epithelial, equatorial, and fiber cells. Primary lens cell cultures were also analyzed. cDNA was generated by reverse transcription of the mRNA portion of the total RNA isolated from each sample. Gene expression data were generated using quantitative real-time reverse transcription PCR. Data were analyzed in terms of cycle threshold number (C_T) and were normalized to endogenous 18S expression. Western blot analyses were carried out to confirm the presence of two critical MMPs. RESULTS. Anterior and equatorial samples were uncontaminated by fiber cells because they showed high expression of α-crystallin genes but low expression of β- and γ-crystallins. The fibers had high expression of these genes and of MIP. MMP genes were expressed at uniformly low levels in the native tissues except for MMP-14 and -15 (MT1- and MT2-MMP, respectively). In fact, MT1-MMP declined in expression from the anterior epithelium to fibers, whereas MT2-MMP increased. The presence of MT1 and MT2-MMP proforms and faster migrating bands, indicating processed or activated forms, was confirmed at the protein level. TIMP genes were uniformly highly expressed in native tissues, with TIMP-3 having the highest expression in the epithelial tissues and TIMP-2 in the fibers. MMP expression was generally elevated in both sets of cultured cells, including MMP-2 and -9. TIMP genes were also relatively highly expressed in the cultured cells. CONCLUSIONS. MMP expression is generally well regulated in native tissues, with relatively low expression of MMPs and high expression of TIMPs. Membrane-type MMPs (MT1 and 2-MMPs) were the most highly expressed; this is important in a tissue with relatively high membrane content but low extracellular space. The striking reciprocal patterns of expression of MT1-MMP and MT2-MMP indicate that these enzymes are of particular significance in lens function.

Original language	English
Pages (from-to)	4192-4199
Number of pages	8
Journal	Investigative Ophthalmology and Visual Science
Volume	48
Issue number	9
DOIs	https://doi.org/10.1167/iovs.06-1371
Publication status	Published - Sept 2007
Externally published	Yes

ASJC Scopus subject areas

Ophthalmology
Sensory Systems
Cellular and Molecular Neuroscience

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10.1167/iovs.06-1371

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@article{9429e405ce0042899321fab0753ef5d0,

title = "MMP and TIMP expression in quiescent, dividing, and differentiating human lens cells",

abstract = "PURPOSE. Matrix metalloproteinases (MMPs) and the tissue inhibitors of the MMPs (TIMPs) have been implicated in lens differentiation, growth, remodeling, and cataract. Hence, a gene expression analysis was undertaken in epithelial and fiber cells dissected from clear human donor lenses. METHODS. The human lens was dissected into three regions: anterior epithelial, equatorial, and fiber cells. Primary lens cell cultures were also analyzed. cDNA was generated by reverse transcription of the mRNA portion of the total RNA isolated from each sample. Gene expression data were generated using quantitative real-time reverse transcription PCR. Data were analyzed in terms of cycle threshold number (CT) and were normalized to endogenous 18S expression. Western blot analyses were carried out to confirm the presence of two critical MMPs. RESULTS. Anterior and equatorial samples were uncontaminated by fiber cells because they showed high expression of α-crystallin genes but low expression of β- and γ-crystallins. The fibers had high expression of these genes and of MIP. MMP genes were expressed at uniformly low levels in the native tissues except for MMP-14 and -15 (MT1- and MT2-MMP, respectively). In fact, MT1-MMP declined in expression from the anterior epithelium to fibers, whereas MT2-MMP increased. The presence of MT1 and MT2-MMP proforms and faster migrating bands, indicating processed or activated forms, was confirmed at the protein level. TIMP genes were uniformly highly expressed in native tissues, with TIMP-3 having the highest expression in the epithelial tissues and TIMP-2 in the fibers. MMP expression was generally elevated in both sets of cultured cells, including MMP-2 and -9. TIMP genes were also relatively highly expressed in the cultured cells. CONCLUSIONS. MMP expression is generally well regulated in native tissues, with relatively low expression of MMPs and high expression of TIMPs. Membrane-type MMPs (MT1 and 2-MMPs) were the most highly expressed; this is important in a tissue with relatively high membrane content but low extracellular space. The striking reciprocal patterns of expression of MT1-MMP and MT2-MMP indicate that these enzymes are of particular significance in lens function.",

author = "Hodgkinson, {Lisa M.} and George Duncan and Lixin Wang and Pennington, {Caroline J.} and Edwards, {Dylan R.} and Wormstone, {I. Michael}",

year = "2007",

month = sep,

doi = "10.1167/iovs.06-1371",

language = "English",

volume = "48",

pages = "4192--4199",

journal = "Investigative Ophthalmology and Visual Science",

issn = "0146-0404",

publisher = "Association for Research in Vision and Ophthalmology Inc.",

number = "9",

}

TY - JOUR

T1 - MMP and TIMP expression in quiescent, dividing, and differentiating human lens cells

AU - Hodgkinson, Lisa M.

AU - Duncan, George

AU - Wang, Lixin

AU - Pennington, Caroline J.

AU - Edwards, Dylan R.

AU - Wormstone, I. Michael

PY - 2007/9

Y1 - 2007/9

N2 - PURPOSE. Matrix metalloproteinases (MMPs) and the tissue inhibitors of the MMPs (TIMPs) have been implicated in lens differentiation, growth, remodeling, and cataract. Hence, a gene expression analysis was undertaken in epithelial and fiber cells dissected from clear human donor lenses. METHODS. The human lens was dissected into three regions: anterior epithelial, equatorial, and fiber cells. Primary lens cell cultures were also analyzed. cDNA was generated by reverse transcription of the mRNA portion of the total RNA isolated from each sample. Gene expression data were generated using quantitative real-time reverse transcription PCR. Data were analyzed in terms of cycle threshold number (CT) and were normalized to endogenous 18S expression. Western blot analyses were carried out to confirm the presence of two critical MMPs. RESULTS. Anterior and equatorial samples were uncontaminated by fiber cells because they showed high expression of α-crystallin genes but low expression of β- and γ-crystallins. The fibers had high expression of these genes and of MIP. MMP genes were expressed at uniformly low levels in the native tissues except for MMP-14 and -15 (MT1- and MT2-MMP, respectively). In fact, MT1-MMP declined in expression from the anterior epithelium to fibers, whereas MT2-MMP increased. The presence of MT1 and MT2-MMP proforms and faster migrating bands, indicating processed or activated forms, was confirmed at the protein level. TIMP genes were uniformly highly expressed in native tissues, with TIMP-3 having the highest expression in the epithelial tissues and TIMP-2 in the fibers. MMP expression was generally elevated in both sets of cultured cells, including MMP-2 and -9. TIMP genes were also relatively highly expressed in the cultured cells. CONCLUSIONS. MMP expression is generally well regulated in native tissues, with relatively low expression of MMPs and high expression of TIMPs. Membrane-type MMPs (MT1 and 2-MMPs) were the most highly expressed; this is important in a tissue with relatively high membrane content but low extracellular space. The striking reciprocal patterns of expression of MT1-MMP and MT2-MMP indicate that these enzymes are of particular significance in lens function.

AB - PURPOSE. Matrix metalloproteinases (MMPs) and the tissue inhibitors of the MMPs (TIMPs) have been implicated in lens differentiation, growth, remodeling, and cataract. Hence, a gene expression analysis was undertaken in epithelial and fiber cells dissected from clear human donor lenses. METHODS. The human lens was dissected into three regions: anterior epithelial, equatorial, and fiber cells. Primary lens cell cultures were also analyzed. cDNA was generated by reverse transcription of the mRNA portion of the total RNA isolated from each sample. Gene expression data were generated using quantitative real-time reverse transcription PCR. Data were analyzed in terms of cycle threshold number (CT) and were normalized to endogenous 18S expression. Western blot analyses were carried out to confirm the presence of two critical MMPs. RESULTS. Anterior and equatorial samples were uncontaminated by fiber cells because they showed high expression of α-crystallin genes but low expression of β- and γ-crystallins. The fibers had high expression of these genes and of MIP. MMP genes were expressed at uniformly low levels in the native tissues except for MMP-14 and -15 (MT1- and MT2-MMP, respectively). In fact, MT1-MMP declined in expression from the anterior epithelium to fibers, whereas MT2-MMP increased. The presence of MT1 and MT2-MMP proforms and faster migrating bands, indicating processed or activated forms, was confirmed at the protein level. TIMP genes were uniformly highly expressed in native tissues, with TIMP-3 having the highest expression in the epithelial tissues and TIMP-2 in the fibers. MMP expression was generally elevated in both sets of cultured cells, including MMP-2 and -9. TIMP genes were also relatively highly expressed in the cultured cells. CONCLUSIONS. MMP expression is generally well regulated in native tissues, with relatively low expression of MMPs and high expression of TIMPs. Membrane-type MMPs (MT1 and 2-MMPs) were the most highly expressed; this is important in a tissue with relatively high membrane content but low extracellular space. The striking reciprocal patterns of expression of MT1-MMP and MT2-MMP indicate that these enzymes are of particular significance in lens function.

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MMP and TIMP expression in quiescent, dividing, and differentiating human lens cells

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