Kevin Howard scite author profile

Neutrophils are thought to be involved in many infectious diseases and have been found in high numbers in the corneas of patients with Acanthamoeba keratitis. Using a Chinese hamster model of keratitis, conjunctival neutrophil migration was manipulated to determine the importance of neutrophils in this disease. Inhibition of neutrophil recruitment was achieved by subconjunctival injection with an antibody against macrophage inflammatory protein 2 (MIP-2), a powerful chemotactic factor for neutrophils which is secreted by the cornea. In other experiments, neutrophils were depleted by intraperitoneal injection of anti-Chinese hamster neutrophil antibody. The inhibition of neutrophils to the cornea resulted in an earlier onset and more severe infection compared to controls. Anti-MIP-2 antibody treatment produced an almost 35% reduction of myeloperoxidase activity in the cornea 6 days postinfection, while levels of endogenous MIP-2 secretion increased significantly. Recruitment of neutrophils into the cornea via intrastromal injections of recombinant MIP-2 generated an initially intense inflammation that resulted in the rapid resolution of the corneal infection. The profound exacerbation of Acanthamoeba keratitis seen when neutrophil migration was inhibited, combined with the rapid clearing of the disease in the presence of increased neutrophils, strongly suggests that neutrophils play an important role in combating Acanthamoeba infections in the cornea.

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Tear IgA and Serum IgG Antibodies Against Acanthamoeba in Patients With Acanthamoeba Keratitis

Alizadeh

Apte

El-Agha

et al. 2001

Cornea

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Resistance of Acanthamoeba castellanii Cysts to Physical, Chemical, and Radiological Conditions

Aksozek

McClellan

Howard

et al. 2002

Journal of Parasitology

161

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Resistance of Acanthamoeba castellanii cysts to disinfection agents, antimicrobial agents, heat, freeze-thawing, ultraviolet radiation (UV), gamma irradiation, and cellulase were evaluated in vitro. Following exposure to different agents, the cysts were removed and cultured for A. castellanii trophozoites for 3-14 days. Solutions containing 20% isopropyl alcohol or 10% formalin effectively killed A. castellanii cysts. Hydrogen peroxide (3%, AOSept Disinfectant) effectively killed A. castellanii cysts after 4 hr of exposure. Polyhexamethylene biguanide (0.02%), clotrimazole (0.1%), or propamidine isethionate (Brolene) were effective in killing A. castellanii cysts in vitro. Acanthamoeba castellanii cysts were resistant to both 250 K rads of gamma irradiation and 800 mJ/cm2 of UV irradiation. Excystment of trophozoites was accelerated after exposure to 10, 100, and, 1,000 units of cellulase. These results suggest that A. castellanii cysts benefit by enhanced survival because of their resistance to very harsh environmental conditions.

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Upregulation of phagocytosis and candidicidal activity of macrophages exposed to the immunostimulant, acemannan

Stuart

Lefkowitz

Lincoln

et al. 1997

International Journal of Immunopharmacology

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Reduction of Liver Metastasis of Intraocular Melanoma by Interferon-β Gene Transfer

Alizadeh

Howard

Mellon

et al. 2003

Invest. Ophthalmol. Vis. Sci.

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Kevin Howard

Exacerbation ofAcanthamoebaKeratitis in Animals Treated with Anti-Macrophage Inflammatory Protein 2 or Antineutrophil Antibodies

Tear IgA and Serum IgG Antibodies Against Acanthamoeba in Patients With Acanthamoeba Keratitis

Resistance of Acanthamoeba castellanii Cysts to Physical, Chemical, and Radiological Conditions

Upregulation of phagocytosis and candidicidal activity of macrophages exposed to the immunostimulant, acemannan

Reduction of Liver Metastasis of Intraocular Melanoma by Interferon-β Gene Transfer

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