HOME HELP FEEDBACK SUBSCRIPTIONS ARCHIVE SEARCH TABLE OF CONTENTS		QUICK SEARCH:   [advanced] Author: Keyword(s): Year:  Vol:  Page:

This Article Abstract Full Text (PDF) Submit a response Alert me when this article is cited Alert me when eLetters are posted Alert me if a correction is posted Citation Map Services Email this article to a friend Similar articles in this journal Similar articles in PubMed Alert me to new issues of the journal Download to citation manager Citing Articles Citing Articles via HighWire Citing Articles via Google Scholar Google Scholar Articles by Rakic, J.-M. Articles by Munaut, C. Search for Related Content PubMed PubMed Citation Articles by Rakic, J.-M. Articles by Munaut, C.

Estrogens Reduce the Expression of YKL-40 in the Retina: Implications for Eye and Joint Diseases

¹From the Department of Ophthalmology, University Hospital, Sart-Tilman, Liège, Belgium; the Laboratories of ²Tumor and Development Biology and ³Neuropathology, University of Liège, Liège, Belgium.

	Abstract

Top Abstract Methods Results Discussion References

 
PURPOSE. To identify modifications in the gene expression profile of the ocular posterior segment in ovariectomized (OVX) mice with and without substitutive estradiol therapy and to select differentially expressed genes that could be relevant to the natural history of human age-related macular degeneration (AMD).

METHODS. Chorioretinal tissues from two groups of 25 treated and untreated OVX mice were analyzed by using cDNA array technology. The expression level of selected genes was confirmed in triplicate by RT-PCR and related to the estrogenic status of the animals. Expression of the YKL-40 gene was further investigated in intact or diseased human retinas and in a murine model of experimental choroidal neovascularization (CNV), using laser pressure catapulting.

RESULTS. Of the approximately 10,000 genes screened, only YKL-40 expression was significantly downregulated by 17-ß-estradiol. YKL-40 was expressed in intact human neural retina and in the RPE. The expression of YKL-40 was upregulated in experimental CNV and in neovascular membranes extracted from patients affected by the exudative form of AMD.

CONCLUSIONS. These observations indicate that YKL-40 expression in the retina is modulated by serum levels of estradiol. This protein could be relevant to the development of AMD and is also a new mediator to take into account when evaluating the broad consequences of hormonal replacement therapy.

Increasing experimental evidence suggests that estrogens are neuroprotective^{6 7 8} and that estrogen replacement therapy may contribute to the prevention or delay the onset of Alzheimer’s disease.⁹ Menopause coincides also with the appearance or worsening of many common arthritic conditions¹⁰ that are associated with increased levels of proinflammatory cytokines, such as interleukin (IL)-1, IL-6, and tumor necrosis factor-.¹¹ Epidemiologic studies reported conflicting results on the protective effect of hormone replacement therapy (HRT) in the development of the neovascular form of AMD.^{12 13} Others studies, however, failed to demonstrate a significant gender difference in the frequency of the disease.¹⁴ A large clinical trial (Women’s Health Initiative Sight Exam Study) investigating whether HRT may influence the development and the course of macular degeneration is under way.

The mechanisms by which 17-ß-estradiol (E2) protects against AMD are not known. A protective effect has been demonstrated in the ischemia–reperfusion injury model in rat retina.¹⁵ E2 enhances the expression of vascular endothelial growth factor (VEGF) and its receptor (VEGFR-2) in bovine retinal endothelial cells in vitro,¹⁶ but this effect has recently been shown to depend on oxygen status in a murine model of retinopathy of prematurity.¹⁷ Ovariectomy has been suggested to disturb Bruch’s membrane turnover in mice fed with a high-fat diet (Alexandridou A, Elliot S, Espinosa D, Hernandez E, Csaky KG, Cousins SW, ARVO Abstract 1200, 2001).

In the present study, we used cDNA microarray technology to profile gene expression changes (10,000 screened genes) in intact posterior segments of ovariectomized (OVX) mice treated or not with E2 pellets. In a second confirmation phase, the expression of selected genes was investigated by quantitative RT-PCR on individual mice retinas and correlated with the estrogen status. E2 supplementation significantly reduced the expression of one gene, YKL-40 (also known as human cartilage glycoprotein 39, HCgp39). YKL-40 is a mammalian glycoprotein member of a family of 18 glysolyl hydrolases related in sequence to chitinases but without chitinase activity.^{18 19} Its function is unknown, but it is thought to be involved in tissue remodeling, acting as a growth factor for connective tissue cells²⁰ and as a potent migration factor for endothelial cells.²¹ Most of the studies regarding YKL-40 have focused on rheumatoid arthritis (RA), because this protein is an articular autoantigen in mice²² (with pathologic effects similar to those with immunization by collagen type II), and its serum levels are clinically correlated with the severity of the disease.^{23 24} Because this glycoprotein has not been previously described in the retina, we studied its expression in human normal retina, in neovascular choroidal membranes extracted from patients with AMD, and in a murine model of experimental choroidal neovascularization (CNV).

	Methods

Top Abstract Methods Results Discussion References

 
Ovariectomized (OVX) Mice
OVX mice (ovariectomy was performed at 6 weeks of age) were purchased from Charles River France (Lyon, France). In the group (n = 25) receiving substitutive hormonal therapy, estrogens were administered through 3-mm subcutaneous pellets containing 1.7 mg E2 (Innovative Research of America, Sarasota, FL). In the control group, OVX mice (n = 25) received implants of a saline-containing pellet. E2 pellets provide continuous release, allowing for a constant level of circulating hormone. The selected pellet delivered 28 µg/d of E2, providing serum concentrations exceeding the usual physiological concentrations in female mice (100 pg/mL) but lower than high-dose estrogen treatment (e.g., anti-tumor therapy).²⁵ Serum levels of E2 were monitored at the end of the study period by radioimmunoassay, according to the manufacturer’s instructions (Immunotech; Westbrook, ME), as previously described.² After 30 days, mice were killed, and the ocular posterior segments (neural retina and RPE-choroid complex) were removed and frozen in liquid nitrogen. In the treated group, the efficiency of HRT was also controlled by means of uterine weight (approximate fivefold increase in the E2 treated group) and histologic evaluation of the endometrium (not shown). Three mice had to be removed from the study group because of defective pellet implantation. For experiments using RT-PCR, a second set of 20 OVX mice (10 in each group) was treated similarly (2 mice were not analyzed in the E2-treated group because of bad pellet implantation). Animal experiments were performed in compliance with the ARVO Statement for the Use of Animals in Ophthalmic and Vision Research.

cDNA Array
Total RNA was isolated from posterior segments (retina and RPE-choroid complex) from OVX control and OVX-E2–treated mice by using an RNA isolation protocol (TRIzol; Sigma, Belgium), as recommended by the manufacturer. The frozen tissues were first pulverized with a dismembrator (B. Braun Biotech International, GmBH, Melsungen, Germany) and homogenized in the extraction reagent. RNA quality was controlled on 1% agarose gel. RNA samples from each group were pooled and then processed by Incyte Genomics (St. Louis, MO) and hybridized to a cDNA array (Mouse UniGene1; Incyte Genomics, Inc.). This array is designed to provide a broad view of the mouse genome and includes targets for 9596 elements with 8985 unique annotated genes and expressed sequence tag (EST) clusters (list available at http://www.incyte.com/expression/easy_to_spot/catalog/txt_files/mouse_unigene1_gene_list.txt). Gene expression levels were measured and displayed using the manufacturer’s software (GEMTools 2.5; Incyte Genomics).

Human Intact and Pathologic Retinas
Eight consecutive submacular CNV specimens were surgically removed (performed by Carel Claes, MD, A.Z Middelheim, Antwerpen, Belgium) during 360° macular translocations performed on patients with exudative AMD (three men, five women; mean age, 77 years; range, 72–83). These patients were not eligible for conventional laser photodynamic therapy because of the presence of occult new vessels or submacular bleeding, or, in the case of one patient, because of a recurrence of the disease. The methods conformed to the Declaration of Helsinki for research involving human subjects. The specimens were snap frozen in liquid nitrogen and stored at -80°C. Ten human male and female donor eyes were also obtained from the Cornea Bank, University of Liège, Belgium, as a source of intact neural retina and RPE-choroid. After removal of the anterior segment structures, 5-mm diameter punches were made in the macular region and in the peripheral retina (to estimate differential expression between the two regions), frozen in liquid nitrogen, and stored at -80°C.

Laser Pressure Catapulting
For laser pressure catapulting (LPC), experimental CNV was induced by laser in C57BL mice (n = 12), as previously described,²⁶ to evaluate the spatial and temporal pattern of YKL-40 expression. The eyes were enucleated at selected intervals after induction (days 3, 6, 14, and 40), embedded in mounting compound (Tissue Tek; Miles Laboratories, Naperville, IL), and frozen in liquid nitrogen. Serial frozen sections (n = 8–10) were mounted directly on 1.35-mm thin polyethylene foil (Palm, Wolfratshausen, Germany), which had been mounted on the glass slide using a robotic technique (Microbeam-Moment; Palm).²⁷ The robot microbeam (Palm) focused the laser (337 nm) on the specimen, catapulting the selected area into the microfuge cap. The entire subretinal CNV area (as shown in Fig. 4C ) and an adjacent intact chorioretinal zone (control) were microdissected separately on frozen sections (10 µm thick). The specimens were covered with 100 µL lysis buffer, and total RNA isolation was performed with an RNA isolation kit (PureScript RNA; BioZym, Landgraaf, The Netherlands) according to the manufacturer’s protocol. Total RNA was dissolved in a 10 µL RNA hydration solution supplied by the manufacturer, and RT-PCR was performed.

View larger version (59K): [in this window] [in a new window]   FIGURE 4. Expression of YKL-40 mRNA in human retina and in CNV. (A) YKL-40 mRNA was present in human normal neural retina (R) and in the RPE-choroid complex (Ch), both in the macular region (I) and in the periphery (O). Age of the donors is given in years with gender. (B) Representative example of YKL-40 mRNA expression in surgically extracted choroidal neovascular membranes of four patients with exudative AMD. Total RNA (10 ng) was subjected to RT-PCR. (C) LPC followed by RT-PCR analysis of YKL-40 expression (with pigmented epithelium-derived growth factor [PEDF] used as an additional control gene on microdissected new choroidal vessels growing in the subretinal space (CNV, delineated by dotted line) and on adjacent (control) intact chorioretinal tissue (R) from days 3 to 40. Multiple bands under YKL-40 or PEDF signals represent multimers of primers. Molecular weights are shown at left (expected size for 28S product is 212 bp; for PEDF, 256 bp; for human YKL-40, 112 bp; and for murine YKL-40 142 bp).

	Results

Top Abstract Methods Results Discussion References

 
Effects of E2 on Chorioretinal mRNA Profile
The mean E2 serum level was 15.08 ± 4.2 pg/mL in OVX-untreated mice and 537 ± 79.7 pg/mL in E2-treated mice, indicating that ovariectomy reduced endogenous circulating E2 concentrations, whereas supplementation with 1.7-mg estradiol pellets restored circulating concentrations of E2 moderately over the physiological range (100 pg/mL).²⁵ Only a minority of the genes tested on the cDNA array showed a noticeable change of their expression after 30 days of substitutive E2 therapy. Less than 1% of tested genes displayed a differential expression ratio of 1.5 or more, and most of them appeared to be upregulated by E2 deficiency (Fig. 1) . The cDNA microarray expression data of selected genes are shown in Table 2 . The largest difference in expression (ratio = 2) was seen for the YKL-40 gene with lower expression in OVX E2-treated mice. The influence of E2 supplementation on YKL-40 expression was confirmed by semiquantitative RT-PCR (in triplicate and with two different couples of oligonucleotides normalized to 28S signal) performed on a second set of animals and related to the presence or absence of E2 supplementation (Fig. 2) . Several genes showing similar expression levels in the E2-treated and untreated groups were assessed in parallel by RT-PCR and used as the negative control (Fig. 3) .

View larger version (14K): [in this window] [in a new window]   FIGURE 1. Frequency of genes exhibiting different levels of expression (in multiples of change) in OVX mice supplemented or not with E2 pellets (increased expressions are shown as negative values).

View larger version (15K): [in this window] [in a new window]   FIGURE 2. Influence of E2 treatment on YKL-40 gene expression in OVX mice. (A) Representative example of YKL-40 mRNA expression in the eye of individual mice. (B) Relative levels of YKL-40 mRNA (densitometric quantification and normalization to the 28S signal) in the E2-treated (+E2) and untreated (-E2) group.

View larger version (10K): [in this window] [in a new window]   FIGURE 3. Confirmation by RT-PCR of the cDNA array results for selected genes (used as negative control). Transthyretin, retinol binding protein (RBP), angiogenin, and VEGF-A mRNA expression levels (densitometric quantification and normalization to 28S signal) in ocular posterior segments of individual mice. There was no statistically significant difference between mean mRNA expression in the E2-treated or untreated OVX mice (P > 0.05, t-test).

YKL-40 Expression Profile in Human and Mouse Neovascular Membranes
YKL-40 expression was detected in normal human posterior segments from different donors (Fig. 4A) . YKL-40 was detected in ocular tissues from patients of different age and gender, regardless of the region of the sample (inside or outside the macula, retina or RPE-choroid complex). YKL-40 mRNA was also detected in all CNV specimens obtained during surgery (Fig. 4B) . Although sharing in common the unfeasibility of conventional treatment, these neovascular membranes had a documented different natural history (size of the lesion, duration of symptoms, previous treatment). To evaluate more precisely the spatial (lesion versus intact adjacent regions) and temporal pattern of YKL-40 expression, RT-PCR analysis was applied to laser-induced murine neovascular choroidal membranes microdissected (Fig. 4C , left) by LPC at different time end points (days 3–40 after laser-induced CNV). When compared with intact adjacent regions, upregulation of YKL-40 mRNA expression was evident in CNV lesions at all end points (Fig. 4C) .

	Discussion

Top Abstract Methods Results Discussion References

 
DNA microarrays are powerful tools that allow for genome-wide gene expression profiling of cells or tissues.³² In this study, we used a cDNA array testing for approximately 10,000 genes to identify modification of the gene expression profile of pooled ocular posterior segments in ovariectomized mice rescued or not by substitutive E2 therapy. In this experimental setting, less than 1% of the genes tested showed noticeable expression changes. Among them, the YKL-40 gene showed the largest expression change, with lower values in OVX E2-treated mice. This observation was confirmed by semiquantitative RT-PCR in a second set of experiments performed on individual mice tissues. YKL-40 gene expression was further studied in normal and pathologic human retinas.

YKL-40 expression has been reported in human RPE, with serial analysis of gene expression technology (SAGE).³³ In the current study, YKL-40 was consistently expressed in normal human eyes both in neural retina and in the RPE-choroid complex. High concentrations of YKL-40 in serum correlates with morbidity in different human diseases such as active rheumatoid arthritis and hepatic fibrosis, as well as with death of recurrent colorectal cancer.^{34 35 36} YKL-40 is produced by monocytes in the media of arteritic vessels, in inflamed synovial membranes, and in atherosclerotic plaques, suggesting a role for YKL-40 in tissue remodeling.^{37 38} In vitro, YKL-40 is one of the most abundant proteins secreted by cultured chondrocytes.³⁹ The regulation of YKL-40 expression, however, is largely unknown. In this study YKL-40 was significantly downregulated by estrogen supplementation in the ocular posterior segment of OVX mice. Furthermore, YKL-40 expression was upregulated both in pathologic human and experimental CNV, although we cannot exclude bias caused by our selecting specimens from patients for whom standard laser therapy could not be used. Taken together with the migratory properties of YKL-40 in endothelial cells,²¹ these data suggest a proangiogenic role of YKL-40 in the development of exudative AMD and could at least partly verify a protective role for estrogen replacement therapy.^{12 13} A direct effect of YKL-40 on angiogenesis in other in vitro and in vivo models, such as corneal pellets or aortic rings, has yet to be evaluated. If a similar regulation were to be demonstrated in the synovium, our results could also provide a putative explanation for the protective effect of estrogens in rheumatoid arthritis, because YKL-40 has been proposed as a candidate autoantigen in this disease,²³ and its serum levels are related to disease activity.²⁵

It is of interest that, in our model of OVX mice, only a limited number of genes were affected by estrogen therapy in the retina. This could be explained by the pooling of samples for cDNA array, which selected only for strong and constant differences of gene expression and minimized individual variations. In particular, the expression of cathepsin D, an aspartic protease highly expressed in human retinal pigment epithelial lysosomes⁴⁰ with transcription classically regulated by estrogens in breast cancer,⁴¹ was not influenced in vivo in the murine retina. Experimental impairment of cathepsin D results in accumulation of rod outer segment debris in the RPE and as been suggested as a murine model of dry AMD.⁴² A similar discrepancy has been reported for endometrial cells and attributed to differential tissue-dependent regulation.⁴³ Individual variations in the level of mRNA expression for a specific gene are evident from the confirmation phase of our study, especially in the OVX untreated group. There was up to a 15-fold modulation of VEGF-A expression between mice of the same group. This could be explained by variations in very low level E2 concentrations (picomolar range), which have been demonstrated to enhance gene expression in different models.⁴⁴ It is also known that for some genes, the mechanism of regulation by estrogens is posttranscriptional rather than at the transcriptional level. This was indeed demonstrated for hepatic apolipoprotein E.⁴⁵ Finally, because the levels of ER- and -ß mRNA were weak in murine posterior segment, we cannot exclude the possibility that HRT could modify other genes in the human retina, in which these receptors are expressed at a higher level.²

This study is obviously a preliminary phase in the understanding of the potential influences of HRT on AMD, and it would be of great interest to evaluate by cDNA microarray HRT-treated and untreated patients, as well as to compare intact and AMD tissue specimens. Our data nevertheless identify for the first time the YKL-40 gene as a potential mediator of estrogens effects both in the normal eye and during the development of CNV.

	Footnotes

 
Supported by grants from Les Amis des Aveugles, Ghlin, Belgium. CM is a research associate and AN a senior research associate from the National Fund for Scientific Research (FNRS), Belgium.

Submitted for publication August 1, 2002; revised August 29 and September 19, 2002; accepted September 25, 2002.

Disclosure: J.-M. Rakic, None; V. Lambert, None; M. Deprez, None; J.-M. Foidart, None; A. Noël, None; C. Munaut, None

The publication costs of this article were defrayed in part by page charge payment. This article must therefore be marked "advertisement" in accordance with 18 U.S.C. 1734 solely to indicate this fact.

Corresponding author: Jean-Marie Rakic, Polyclinique d’Ophtalmologie, Centre Hospitalier Universitaire, Sart-Tilman, B-4000 Liège, Belgium; jmrakic{at}chu.ulg.ac.be.

	References

Top Abstract Methods Results Discussion References

 

1. Ogueta, SB, Schwartz, SD, Yamashita, CK, Farber, DB. (1999) Estrogen receptor in the human eye: influence of gender and age on gene expression Invest Ophthalmol Vis Sci 40,1906-1911[Abstract/Free Full Text]
2. Munaut, C, Lambert, V, Noel, A, et al (2001) Presence of oestrogen receptor type beta in human retina Br J Ophthalmol 85,877-882[Abstract/Free Full Text]
3. Bigsby, RM, Cardenas, H, Caperell-Grant, A, Grubbs, CJ. (1999) Protective effects of estrogen in a rat model of age-related cataracts Proc Natl Acad Sci USA 96,9328-9332[Abstract/Free Full Text]
4. Davis, VL, Chan, CC, Schoen, TJ, Couse, JF, Chader, GJ, Korach, KS. (2002) An estrogen receptor repressor induces cataract formation in transgenic mice Proc Natl Acad Sci USA 99,9427-9432[Abstract/Free Full Text]
5. Benitez del Castillo, JM, del Rio, T, Garcia-Sanchez, J. (1997) Effects of estrogen use on lens transmittance in postmenopausal women Ophthalmology 104,970-973[Medline][Order article via Infotrieve]
6. Behl, C. (2002) Oestrogen as a neuroprotective hormone Nat Rev Neurosci 6,433-442[CrossRef]
7. Behl, C, Widmann, M, Trapp, T, Holsboer, F. (1995) 17-beta Estradiol protects neurons from oxidative stress-induced cell death in vitro Biochem Biophys Res Commun 216,473-482[CrossRef][Medline][Order article via Infotrieve]
8. Kadish, I, Van Groen, T. (2002) Low levels of estrogen significantly diminish axonal sprouting after entorhinal cortex lesions in the mouse J Neurosci 22,4095-4102[Abstract/Free Full Text]
9. Tang, MX, Jacobs, D, Stern, Y, et al (1996) Effect of oestrogen during menopause on risk and age at onset of Alzheimer’s disease Lancet 348,429-432[CrossRef][Medline][Order article via Infotrieve]
10. Wluka, AE, Cicuttini, FM, Spector, TD. (2000) Menopause, oestrogens and arthritis Maturitas 35,183-199[CrossRef][Medline][Order article via Infotrieve]
11. Pfeilschifter, J, Koditz, R, Pfohl, M, Schatz, H. (2002) Changes in proinflammatory cytokine activity after menopause Endocr Rev 23,90-119[Abstract/Free Full Text]
12. . The Eye Disease Case-Control Study Group. (1992) Risk factors for neovascular age-related macular degeneration Arch Ophthalmol 110,1701-1708[Abstract/Free Full Text]
13. Smith, W, Mitchell, P, Wang, JJ. (1997) Gender, oestrogen, hormone replacement and age-related macular degeneration: results from the Blue Mountains Eye Study Aust NZ J Ophthalmol 25(suppl 1),S13-S15
14. Smith, W, Assink, J, Klein, R, Mitchell, P, et al (2001) Risk factors for age-related macular degeneration: pooled findings from three continents Ophthalmology 108,697-704[CrossRef][Medline][Order article via Infotrieve]
15. Nonaka, A, Kiryu, J, Tsujikawa, A, et al (2000) Administration of 17beta-estradiol attenuates retinal ischemia-reperfusion injury in rats Invest Ophthalmol Vis Sci 41,2689-2696[Abstract/Free Full Text]
16. Suzuma, I, Mandai, M, Takagi, H, et al (1999) 17-ß-Estradiol increases VEGF receptor-2 and promotes DNA synthesis in retinal microvascular endothelial cells Invest Ophthalmol Vis Sci 40,2122-2129[Abstract/Free Full Text]
17. Miyamoto, N, Mandai, M, Takagi, H, et al (2002) Contrasting effect of estrogen on VEGF induction under different oxygen status and its role in murine ROP Invest Ophthalmol Vis Sci 43,2007-2014[Abstract/Free Full Text]
18. Hakala, BE, White, C, Recklies, AD. (1993) Human cartilage gp-39, a major secretory product of articular chondrocytes and synovial cells, is a mammalian member of a chitinase protein family J Biol Chem 268,25803-25810[Abstract/Free Full Text]
19. Rehli, M, Krause, SW, Andreesen, R. (1997) Molecular characterization of the gene for human cartilage gp-39 (CHI3L1), a member of the chitinase protein family and marker for late stages of macrophage differentiation Genomics 43,221-225[CrossRef][Medline][Order article via Infotrieve]
20. De Ceuninck, F, Gaufillier, S, Bonnaud, A, Sabatini, M, Lesur, C, Pastoureau, P. (2001) YKL-40 (cartilage gp-39) induces proliferative events in cultured chondrocytes and synoviocytes and increases glycosaminoglycan synthesis in chondrocytes Biochem Biophys Res Commun 285,926-931[CrossRef][Medline][Order article via Infotrieve]
21. Malinda, KM, Ponce, L, Kleinman, HK, Shackelton, LM, Millis, AJ. (1999) Gp38K, a protein synthesized by vascular smooth muscle cells, stimulates directional migration of human umbilical vein endothelial cells Exp Cell Res 250,168-173[CrossRef][Medline][Order article via Infotrieve]
22. Verheijden, GF, Rijnders, AW, Bos, E, et al (1997) Human cartilage glycoprotein-39 as a candidate autoantigen in rheumatoid arthritis Arthritis Rheum 40,1115-1125[Medline][Order article via Infotrieve]
23. Vos, K, Steenbakkers, P, Miltenburg, AM, et al (2000) Raised human cartilage glycoprotein-39 plasma levels in patients with rheumatoid arthritis and other inflammatory conditions Ann Rheum Dis 59,544-548[Abstract/Free Full Text]
24. Johansen, JS, Stoltenberg, M, Hansen, M, et al (1999) Serum YKL-40 concentrations in patients with rheumatoid arthritis: relation to disease activity Rheumatology 38,618-626[Abstract/Free Full Text]
25. Bourassa, PAK, Milos, PM, Gaynor, BJ, Breslow, JL, Aiello, RJ. (1996) Estrogen reduces atherosclerotic lesion development in apolipoprotein E-deficient mice Proc Natl Acad Sci USA 93,10022-10027[Abstract/Free Full Text]
26. Lambert, V, Munaut, C, Noel, A, et al (2001) Influence of plasminogen activator inhibitor type I on choroidal neovascularization FASEB J 15,1021-1027[Abstract/Free Full Text]
27. Bohm, M, Wieland, I, Schutze, K, Rubben, H. (1997) Microbeam MOMeNT: non-contact laser microdissection of membrane-mounted native tissue Am J Pathol 151,63-67[Abstract]
28. Meri, S, Morgan, BP, Davies, A, et al (1990) Human protectin (CD59), an 18,000–20,000 MW complement lysis restricting factor, inhibits C5b-8 catalysed insertion of C9 into lipid bilayers Immunology 71,1-9[Medline][Order article via Infotrieve]
29. Mullins, RF, Russell, SR, Anderson, DH, Hageman, GS. (2000) Drusen associated with aging and age-related macular degeneration contain proteins common to extracellular deposits associated with atherosclerosis, elastosis, amyloidosis, and dense deposit disease FASEB J 14,835-846[Abstract/Free Full Text]
30. Magabo, KS, Horwitz, J, Piatigorsky, J, Kantorow, M. (2000) Expression of betaB(2)-crystallin mRNA and protein in retina, brain, and testis Invest Ophthalmol Vis Sci 41,3056-3060[Abstract/Free Full Text]
31. Xu, ZP, Tsuji, T, Riordan, JF, Hu, GF. (2002) The nuclear function of angiogenin in endothelial cells is related to rRNA production Biochem Biophys Res Commun 294,287-292[CrossRef][Medline][Order article via Infotrieve]
32. Duggan, DJ, Bittner, M, Chen, Y, Meltzer, P, Trent, JM. (1999) Expression profiling using cDNA microarrays Nat Genet 1(suppl),10-14
33. Sharon, D, Blackshaw, S, Cepko, CL, Dryja, TP. (2002) Profile of the genes expressed in the human peripheral retina, macula, and retinal pigment epithelium determined through serial analysis of gene expression (SAGE) Proc Natl Acad Sci USA 99,315-320[Abstract/Free Full Text]
34. Matsumoto, T, Tsurumoto, T. (2001) Serum YKL-40 levels in rheumatoid arthritis: correlations between clinical and laboratory parameters Clin Exp Rheumatol 19,655-660[Medline][Order article via Infotrieve]
35. Johansen, JS, Christoffersen, P, Moller, S, et al (2000) Serum YKL-40 is increased in patients with hepatic fibrosis J Hepatol 32,911-920[CrossRef][Medline][Order article via Infotrieve]
36. Cintin, C, Johansen, JS, Christensen, IJ, Price, PA, Sorensen, S, Nielsen, HJ. (1999) Serum YKL-40 and colorectal cancer Br J Cancer 79,1494-1499[CrossRef][Medline][Order article via Infotrieve]
37. Johansen, JS, Baslund, B, Garbarsch, C, et al (1999) YKL-40 in giant cells and macrophages from patients with giant cell arteritis Arthritis Rheum 42,2624-2630[CrossRef][Medline][Order article via Infotrieve]
38. Boot, RG, van Achterberg, TA, van Aken, BE, et al (1999) Strong induction of members of the chitinase family of proteins in atherosclerosis: chitotriosidase and human cartilage gp-39 expressed in lesion macrophages Arterioscler Thromb Vasc Biol 19,687-694[Abstract/Free Full Text]
39. Johansen, JS, Olee, T, Price, PA, Hashimoto, S, Ochs, RL, Lotz, M. (2001) Regulation of YKL-40 production by human articular chondrocytes Arthritis Rheum 44,826-837[CrossRef][Medline][Order article via Infotrieve]
40. Rakoczy, PE, Lai, CM, Baines, M, Di Grandi, S, Fitton, JH, Constable, IJ. (1997) Modulation of cathepsin D activity in retinal pigment epithelial cells Biochem J 324,935-940
41. Rochefort, H, Chalbos, D, Cunat, S, Lucas, A, Platet, N, Garcia, M. (2001) Estrogen regulated proteases and antiproteases in ovarian and breast cancer cells J Steroid Biochem Mol Biol 76,119-124[CrossRef][Medline][Order article via Infotrieve]
42. Zhang, D, Lai, MC, Constable, IJ, Rakoczy, PE. (2002) A model for a blinding eye disease of the aged Biogerontology 3,61-66[CrossRef][Medline][Order article via Infotrieve]
43. Miralles, F, Gaudelet, C, Cavailles, V, Rochefort, H, Augereau, P. (1994) Insensitivity of cathepsin D gene to estradiol in endometrial cells is determined by the sequence of its estrogen responsive element Biochem Biophys Res Commun 203,711-718[CrossRef][Medline][Order article via Infotrieve]
44. Sobel, MI, Winkel, CA, Macy, LB, Liao, P, Bjornsson, TD. (1995) The regulation of plasminogen activators and plasminogen activator inhibitor type 1 in endothelial cells by sex hormones Am J Obstet Gynecol 173,801-808[CrossRef][Medline][Order article via Infotrieve]
45. Srivasta, RAK, Srivasta, N, Averna, M, et al (1997) Estrogen up-regulates apolipoprotein E (ApoE) gene expression by increasing ApoE mRNA in the translating pool via the estrogen receptor -mediated pathway J Biol Chem 272,33360-33366[Abstract/Free Full Text]

This article has been cited by other articles:

				D. Feskanich, E. Cho, D. A. Schaumberg, G. A. Colditz, and S. E. Hankinson Menopausal and Reproductive Factors and Risk of Age-Related Macular Degeneration Arch Ophthalmol, April 1, 2008; 126(4): 519 - 524. [Abstract] [Full Text] [PDF]

This Article Abstract Full Text (PDF) Submit a response Alert me when this article is cited Alert me when eLetters are posted Alert me if a correction is posted Citation Map Services Email this article to a friend Similar articles in this journal Similar articles in PubMed Alert me to new issues of the journal Download to citation manager Citing Articles Citing Articles via HighWire Citing Articles via Google Scholar Google Scholar Articles by Rakic, J.-M. Articles by Munaut, C. Search for Related Content PubMed PubMed Citation Articles by Rakic, J.-M. Articles by Munaut, C.