Cellular level characterization of capillary regression in inflammatory angiogenesis using an in vivo corneal model

Peebo, Beatrice Bourghardt; Traneus-Röckert, Catharina; Lagali, Neil

doi:10.1007/s10456-011-9223-3

Cited by 30 publications

(44 citation statements)

References 38 publications

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“…The microscope was equipped with a 63x/0.95 NA water-immersion objective (Zeiss, Oberkochen, Germany), that provides an en face view of a 400 µm x 400 µm corneal area at a selectable corneal depth. The IVCM imaging technique has been described in detail elsewhere (Bourghardt Peebo et al, 2011;Peebo et al, 2011Peebo et al, ,2010. The focal depth of the HRT3 was initially adjusted to image the corneal epithelial surface, and the lateral and transverse microscope alignments were adjusted to locate the suture in the real-time image display window.…”

Section: In Vivo Confocal Microscopymentioning

confidence: 99%

“…Digital images were recorded at 5 frames/s while lateral, transverse, and axial controls were adjusted during image capture to locate and follow the path of cells or vessels from the limbus to the suture area. IVCM has been shown to be a valuable tool for imaging of various cells in transparent tissue, noninvasively, in a time-lapse manner, without the need for cell labeling (Bourghardt Peebo et al, 2011;Peebo et al, 2011Peebo et al, ,2010.…”

Section: In Vivo Confocal Microscopymentioning

confidence: 99%

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Early effects of dexamethasone and anti-VEGF therapy in an inflammatory corneal neovascularization model

Mirabelli

Peebo

Xeroudaki

et al. 2014

Experimental Eye Research

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Inflammatory angiogenesis is the pathogenic mechanism of various sight-threatening eye diseases, among them corneal neovascularization. Current treatment options include steroids which have undesirable side effects, or anti-VEGF which has only limited efficacy. In an inflammatory environment, however, angiogenesis can be stimulated by numerous factors not directly targeted by anti-VEGF therapy. The aim of this study was to induce corneal inflammation leading to angiogenesis, and investigate the early, differential effects of steroid and anti-VEGF therapy at the cellular, tissue, and gene expression levels. Fifty-two Wistar rats received a single intrastromal corneal suture to induce a controlled inflammatory angiogenic response. Rats were subsequently treated with dexamethasone, rat specific anti-VEGF, or goat IgG (control), topically 4 times daily for 7 days. In vivo confocal microscopy of the cornea was performed longitudinally from 5 h up to 7 d to investigate morphology at the cellular and tissue-level. In vivo photographic vessel analysis and immunohistochemistry were also performed. RT-PCR for VEGF-A, FGF-2, IL-6, TNF-alpha, CXCL2, CCL2, CCL3 and DLL4 was performed at 24 h, and for VEGF-A, IL-6, TNF-alpha, FGF-2, CXCL2, CCL2, and CCL3 at 7 days. Early infiltration of CD11b + myeloid cells into the cornea at 5 h post-suture was delayed by both treatments relative to controls; however neither treatment was able to suppress accumulation of myeloid cells at day 2 or 7. Limbal vessel dilation was inhibited at 5 h by both treatments, but only dexamethasone showed sustained effect until day 2. Early macrophage recruitment was also suppressed by dexamethasone (but not by anti-VEGF) until day 2. Dexamethasone furthermore suppressed corneal neovascularization at day 7 by over 90%, whereas suppression by anti-VEGF was 14%. Despite differential suppression of vessel dilation, macrophage recruitment, and vascular invasion, anti-VEGF and dexamethasone both down-regulated VEGF-A and IL-6 expression at 24 h with sustained effect to 7 d. They also both down regulated FGF-2 and TNF-alpha at 24 h and CCL2 at 7 d. In conclusion, anti-angiogenic treatments influence early, pre-angiogenic tissue activity such as limbal vessel dilation, inflammatory cell infiltration of the stroma, and macrophage recruitment. Importantly, the differential effects of steroids and anti-VEGF treatment in suppressing neovascular growth could not be attributed to differential inhibition of several major angiogenic and inflammatory factors in the early pre-sprouting phase, including IL-6, VEGF-A, FGF-2, TNF-alpha, CCL2, CCL3, CXCL2, or DLL4.

Funding Agencies|Crown Princess Margaretas Foundation; County Council of Ostergotland; Swedish Research Council [2012-2472]

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Section: In Vivo Confocal Microscopymentioning

confidence: 99%

Section: In Vivo Confocal Microscopymentioning

confidence: 99%

Early effects of dexamethasone and anti-VEGF therapy in an inflammatory corneal neovascularization model

Mirabelli

Peebo

Xeroudaki

et al. 2014

Experimental Eye Research

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Funding Agencies|Crown Princess Margaretas Foundation; County Council of Ostergotland; Swedish Research Council [2012-2472]

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“…IVCM has also been used for clinical diagnosis of pathology of the cornea and as a screening/monitoring tool for patients undergoing treatment [112][113][114][115]. Other applications are distinguishing different inflammatory cell subtypes in corneal inflammation, and feature recognition for diagnosis, such as acanthamoeba and fungal keratitis.…”

Section: In Vivo Confocal Microscopymentioning

confidence: 99%

Surgical outcomes of phototherapeutic keratectomy on Epithelial basement membrane dystrophy, and the characterisation of Bowman's Layer

Germundsson¹

2014

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“…At day 7 after suture placement, the cornea was fully vascularized from the limbus to the suture, as previously depicted. 16 Both prior to, and at 1, 4, 7, 14, and 21 days after the initial surgery, rats were anesthetized and laser scanning in vivo confocal microscopy (IVCM; HRT3-RCM, Heidelberg Engineering, Heidelberg, Germany) of the corneas was performed.…”

Section: Rat Model Of Suture-induced Inflammatory Corneal Neovascularmentioning

confidence: 99%

Anin VivoMethod for Visualizing Flow Dynamics of Cells within Corneal Lymphatics

Peebo

Lagali

2013

Lymphatic Research and Biology

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Background: Monitoring the trafficking of specific cell populations within lymphatics could improve our understanding of processes such as transplant rejection and cancer metastasis. Current methods, however, lack appropriate image resolution for single-cell analysis or are incompatible with in vivo and longitudinal monitoring of lymphatics in their native state. We therefore sought to achieve high-resolution live imaging of the dynamic behavior of cells within lymph vessels in the rat cornea. Methods/Results: Inflammatory angiogenesis was induced by suture placement in corneas of Wistar rats. Preand up to 3 weeks post-induction, corneas were noninvasively examined by laser-scanning in vivo corneal confocal microscopy (IVCM) using only endogenous contrast. Lymph vessels and the cells harbored therein were documented by still images, real-time video, and 3D confocal stack reconstruction of live tissue. In vivo, conjunctival and corneal lymphatics were morphologically distinct, those with corneal location being onequarter the diameter of those in the conjunctiva ( p < 0.001). Cells were recruited to initially empty pre-existing lymph vessels during the first day of inflammation and maintained a dense occupation of vessels for up to 7 days. A diverse population of cells (diameter range: 1.5-27.5 lm) with varying morphology was observed, and exhibited variable flow patterns and were transported singly and in clusters of at least 2-9 adherent cells. Conclusions: The in vivo microscopic technique presented enables lymph vessels and cell trafficking to be studied in high resolution in a minimally-perturbed physiologic milieu.

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Cellular level characterization of capillary regression in inflammatory angiogenesis using an in vivo corneal model

Cited by 30 publications

References 38 publications

Early effects of dexamethasone and anti-VEGF therapy in an inflammatory corneal neovascularization model

Early effects of dexamethasone and anti-VEGF therapy in an inflammatory corneal neovascularization model

Surgical outcomes of phototherapeutic keratectomy on Epithelial basement membrane dystrophy, and the characterisation of Bowman's Layer

Anin VivoMethod for Visualizing Flow Dynamics of Cells within Corneal Lymphatics

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