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Dive into the research topics where Eva Stodulkova is active.

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Featured researches published by Eva Stodulkova.


FEBS Letters | 2001

Evidence of a tissue-restricting DNA regulatory element in the mouse IRBP promoter

Jeffrey H. Boatright; Barry E. Knox; K.M. Jones; Eva Stodulkova; Ht Nguyen; S.A. Padove; D.E. Borst; John M. Nickerson

The expression of interphotoreceptor retinoid binding protein (IRBP) is limited to photoreceptor cells of the retina and pinealocytes of the pineal gland. We sought to define cis‐elements of the mouse IRBP 5′ flanking region that are required for this restricted activity. In vitro transient transfections of retinoblastoma and neuroblastoma cells and in vivo experiments with transgenic Xenopus laevis indicate that −1783/+101 and −156/+101 IRBP gene fragments directed expression predominantly to the retina and pineal, with minor neuronal expression elsewhere. In contrast, a −70/+101 fragment was less restrictive in controlling expression, exhibiting activity not only in retina, but also in forebrain, hindbrain, spinal cord, and motor neurons innervating gills.


Vision Research | 2002

The effect of retinoids and butyrate on the expression of CRX and IRBP in retinoblastoma cells.

Jeffrey H. Boatright; Eva Stodulkova; Vt Do; S.A. Padove; Ht Nguyen; D.E. Borst; John M. Nickerson

We sought to determine whether differentiation agents such as retinoids and butyrate regulate transcript levels of interphotoreceptor retinoid binding protein (IRBP) and cone rod homeobox (CRX), a homeodomain transcription factor that regulates IRBP promoter activity. WERI-Rb1 retinoblastoma cells were treated with all-trans retinol, all-trans retinoic acid, or butyrate. IRBP and CRX mRNA levels were determined by quantitative RT-PCR. Butyrate at low concentrations increased both mRNA levels but suppressed them at higher concentrations. Retinoic acid had minimal effects. Retinol increased CRX mRNA over four fold. IRBP and CRX transcript levels are sensitive to butyrate and CRX expression is sensitive to retinol.


Current Eye Research | 2001

Extra-hepatic expression of serum albumin mRNA in mouse retina

Christopher S. Dodson; Kalpana Rengarajan; Hilary D. Gewant; Eva Stodulkova; Ha T. Nguyen; Jeffrey H. Boatright; John M. Nickerson

Purpose. In some mammals, serum albumin protein exists in the interphotoreceptor space (IPS), the space between photoreceptor cells and the retinal pigment epithelium. Serum albumin is synthesized largely in the liver, though low levels of extra-hepatic expression have been documented in several other tissues, including fetal rat kidney, pancreas, lung, and heart. The purpose of this study was to investigate whether serum albumin protein and mRNA are found in mouse retina. Methods. Using albumin rabbit antibodies and HRP goat anti-(rabbit IgG), we performed immunoassays on mouse IPS washes to detect the presence of serum albumin protein. Protein extracts from IPS washes were subjected to Affigel Blue chromatography. This resin has an affinity for serum albumin. Reverse transcription-polymerase chain reaction (RT-PCR) of retina total RNA was performed to search for albumin mRNA. Also, real-time reverse transcription polymerase chain reaction (RT-RT-PCR) was employed to look at the levels of expression in different age groups. Results. A constituent of the IPS washes specifically bound and eluted from Affigel Blue column, suggesting that the washes contained serum albumin. SDS PAGE revealed that the size of the constituent was 67 kDa, the size of serum albumin. This 67 kDa band reacted with mouse serum antibody. An RT-PCR amplified fragment of serum albumin mRNA from retina displayed the expected size. The sequence of this fragment is identical to authentic serum albumin cDNA sequence. RPE and choroid were negative for serum albumin mRNA. However, rd1 - /rd1 - retina was positive, suggesting that at least some serum albumin is synthesized in the inner layers of the retina. RT-RT-PCR showed that serum albumin mRNA levels in whole retina reached a maximum at about postnatal day 15 and gradually decreased to about one-sixth of maximum at 12 months age. Conclusions. Serum albumin protein and mRNA were found in mouse IPS and retina, suggesting that the protein is synthesized in the retina. The previously demonstrated ability of serum albumin to bind fatty acids and retinoids and its presence in the mouse IPS suggest a role for serum albumin in transporting retinoids in the retina or IPS, especially at young ages when concentrations appear greatest.


Brain Research | 2001

Endogenous CRX expression and IRBP promoter activity in retinoblastoma cells

Jeffrey H. Boatright; Diane E. Borst; Eva Stodulkova; John M. Nickerson

PURPOSE To determine whether antisense oligonucleotides (AODNs) targeted against CRX, a photoreceptor-specific trans-acting factor, suppress CRX expression and interphotoreceptor retinoid binding protein (IRBP) promoter activity. METHODS Cultures of human retinoblastoma cells were transfected with chloramphenicol acetyltransferase (CAT) reporter plasmids containing a mouse IRBP promoter and AODNs directed against CRX. RT-PCR using primers specific to CRX, OTX2, GAPDH, or RNase H was conducted on total RNA isolated from retinoblastoma cells at various times following transfection with AODNs. RESULTS Transfection of retinoblastoma cells with IRBP promoter CAT constructs alone produced high activity. Co-transfection with AODNs suppressed IRBP promoter activity in a concentration-dependent manner, with half-maximal effect produced at about 2 nM AODN concentration. Transfection with CAT constructs containing an SV40 promoter produced high activity that was unaffected by co-transfection with AODNs. RT-PCR products were obtained for all target sequences. CRX RT-PCR product from cells transfected with AODNs was greatly diminished following transfection with an AODN whereas control transcripts, including that of OTX2, were relatively unaffected. CONCLUSIONS The CRX-specific AODNs specifically and potently suppressed CRX expression and IRBP promoter activity, as measured by RT-PCR and transient transfection assays, respectively. Little or no effect was seen on controls. These data suggest that endogenous CRX is required for IRBP promoter activity in retinoblastoma cells.


Molecular Vision | 2007

Single-stranded oligonucleotide-mediated in vivo gene repair in the rd1 retina

Charlotte Andrieu-Soler; M. Halhal; Jeffrey H. Boatright; S.A. Padove; John M. Nickerson; Eva Stodulkova; Rachael E. Stewart; Vincent T. Ciavatta; M. Doat; Jean-Claude Jeanny; Therese de Bizemont; Florian Sennlaub; Yves Courtois; Francine Behar-Cohen


Current Eye Research | 2001

Structural characterization and comparison of promoter activity of mouse and bovine interphotoreceptor retinoid-binding protein (IRBP) gene 5' flanking regions in WERI, Y79, chick retina cells, and transgenic mice

Diane E. Borst; Jeffrey H. Boatright; Jing-Sheng Si; Eva Stodulkova; Nancy Remaley; Luke A. Pallansch; John M. Nickerson


Investigative Ophthalmology & Visual Science | 2007

Critical Confirmation of Oligonucleotide-Induced Gene Repair in the rd1 Mouse

Jeffrey H. Boatright; Vincent T. Ciavatta; Rachael E. Stewart; John M. Nickerson; M.J. Phillips; Eva Stodulkova; Charlotte Andrieu-Soler; M. Doat; M. Halhal; Francine Behar-Cohen


Investigative Ophthalmology & Visual Science | 2003

Partial Purification and Characterization of a Mammalian IRBP Tissue Restricting Factor

Kalpana Rengarajan; Eva Stodulkova; Jeffrey H. Boatright; John M. Nickerson


Investigative Ophthalmology & Visual Science | 2002

Identification of a mammalian IRBP tissue restricting transcription factor by EMSA and UV Photo-crosslinking and SDS-PAGE

Kalpana Rengarajan; Eva Stodulkova; Vt Do; Jeffrey H. Boatright; John M. Nickerson


Investigative Ophthalmology & Visual Science | 2002

Initial Investigation of Gene Repair in Ocular Tissues

Rk Shuler; Jeffrey H. Boatright; Eva Stodulkova; Kalpana Rengarajan; S.A. Padove; John M. Nickerson

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Diane E. Borst

Uniformed Services University of the Health Sciences

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