Antimicrobial efficacy of corneal cross-linking in vitro and in vivo for Fusarium solani: a potential new treatment for fungal keratitis

Ziqian Zhu; Hongmin Zhang; Juan Yue; Susu Liu; Zhijie Li; Liya Wang

doi:10.1186/s12886-018-0727-0

Antimicrobial efficacy of corneal cross-linking in vitro and in vivo for Fusarium solani: a potential new treatment for fungal keratitis

BMC Ophthalmol. 2018 Mar 2;18(1):65. doi: 10.1186/s12886-018-0727-0.

Authors

Ziqian Zhu¹, Hongmin Zhang¹, Juan Yue¹, Susu Liu¹, Zhijie Li², Liya Wang³

Affiliations

¹ People's Hospital of Zhengzhou University and Henan Provincial People's Hospital, Henan Eye Institute, Henan Eye Hospital, Zhengzhou, 450003, China.
² Department of Pediatrics, Baylor College of Medicine, Houston, TX, USA.
³ People's Hospital of Zhengzhou University and Henan Provincial People's Hospital, Henan Eye Institute, Henan Eye Hospital, Zhengzhou, 450003, China. wangliya_55@126.com.

Abstract

Background: Fungal keratitis is one of the major causes of visual impairment worldwide. However, the effectiveness of corneal collagen cross-linking (CXL) for fungal keratitis remains controversial. In this study, we developed an in vitro and an in vivo models to assess the efficacy of CXL for Fusarium keratitis.

Methods: The effect of in vitro CXL fungicidal was evaluated on the cultures of Fusarium solani which were exposed to irradiation for different durations. Viability of fungal was appraised under four conditions: no treatment (control); CXL: UVA (365 nm)/riboflavin; riboflavin and UVA (365 nm). Each batch of sterile plate culture was irradiated for different CXL durations. The in vivo Therapeutic effect was studied on a mouse keratitis model. The animals were divided randomly into three groups: group A with no treatment (control); Group B with CXL treatment for two minutes and group C with CXL treatment for three minutes. The CXL procedure was performed 24 h post inoculation in each group. All mice with corneal involvement were scored daily for 7 days and 10 days after infection. Corneals were extracted at various time points for quantitative fungal recovery. Histological evaluations were conducted to calculate the number of polymorphonuclear cells.

Results: Viability of fungal decreased significantly in CXL group with 30-min irradiation compared with that in control, riboflavin and UVA groups (P < 0.01). The colony-forming units (CFUs) of fungal solutions in culture significantly decreased with CXL treatment (P < 0.05). Clinical scores, corneal lesion, corneal opacity, neovascularization and the depth of ulceration scores in group B and group C were remarkably lower than that in group A (P < 0.05, P = 0.001, P = 0.001, P = 0.034 and P = 0.025 respectively). Scores of group C were much lower than that in group B. Histological revealed that destruction of corneal collagen fibers and infiltration of inflammatory cells into corneal tissue in group B and group C were much lower than that in group A.

Conclusions: We believe that CXL treatment may be applied to fungal keratitis, therapeutic efficacy will improve with longer treatment duration.

Keywords: Antifungal therapeutic use; Corneal collagen cross-linking; Fungal keratitis; Fusarium solani; Mice.

MeSH terms

Animals
Anti-Infective Agents / therapeutic use*
Collagen / metabolism
Colony Count, Microbial
Corneal Stroma / metabolism*
Corneal Ulcer / drug therapy*
Corneal Ulcer / metabolism
Corneal Ulcer / microbiology
Cross-Linking Reagents*
Disease Models, Animal
Eye Infections, Fungal / drug therapy*
Eye Infections, Fungal / metabolism
Eye Infections, Fungal / microbiology
Fusariosis / drug therapy*
Fusariosis / metabolism
Fusariosis / microbiology
Fusarium / drug effects*
Fusarium / isolation & purification
Male
Mice
Mice, Inbred C57BL
Photosensitizing Agents / therapeutic use
Riboflavin / therapeutic use
Ultraviolet Rays

Substances

Anti-Infective Agents
Cross-Linking Reagents
Photosensitizing Agents
Collagen
Riboflavin

Abstract

MeSH terms

Substances

Grants and funding