| Literature DB >> 22937882 |
Norihiko Kanaguchi1, Naoki Narisawa, Tatsuro Ito, Yosuke Kinoshita, Yasuka Kusumoto, Osamu Shinozuka, Hidenobu Senpuku.
Abstract
BACKGROUND: Candida albicans is a dimorphic fungus that is part of the commensal microbial flora of the oral cavity. When the host immune defenses are impaired or when the normal microbial flora is disturbed, C. albicans triggers recurrent infections of the oral mucosa and tongue. Recently, we produced NOD/SCID.e2f1-/- mice that show hyposalivation, decrease of salivary protein flow, lack IgA and IgG in saliva, and have decreased NK cells. Our objective was to characterize C. albicans infection and biofilm formation in mice.Entities:
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Year: 2012 PMID: 22937882 PMCID: PMC3497864 DOI: 10.1186/1472-6831-12-36
Source DB: PubMed Journal: BMC Oral Health ISSN: 1472-6831 Impact factor: 2.757
Figure 1Observation of yeast and hyphal forms, and colony numbers after inoculation. C. albicans yeast and hyphal forms were taken pictures in microscope after incubation of them in YPD and RPMI1640 with 5% FBS (A). The colonization was observed on the YPD agar and BHI agar plates poured swab samples from oral cavity of NOD/SCID.e2f1−/− mice fed 1% sucrose water at 60 min after the inoculation (B). White and black arrow indicated C. albicans and indigenous microorganism colony respectively. These colonies were taken pictures in the stereoscopic microscope. Data were representative in three independent assays. Samples were swabbed from the oral cavities of four 4-month-old female NOD/SCID.e2f1+/+ and NOD/SCID.e2f1−/− mice at 30, 60, and 90 minutes after inoculation using the yeast form. Samples swabbed in mice fed water (C) or 1% sucrose water (D) overnight before inoculation were poured on YPD agar. Samples swabbed in mice fed water (E) or 1% water (F) before inoculation were poured on BHI agar. CFU data were obtained from three independent experiments with four mice from each strain. Values are expressed as the means ± standard deviations (SDs) of the data. Asterisks show significant differences (*P <0.05) in C and D and significant differences (** <0.05) between water (E) and 1% sucrose water (F) for drinking.
Figure 2Comparison of the yeast form and hyphal form in colony numbers of Samples swabbed from the oral cavities at 60 minutes after inoculation of the yeast form or hyphal form in four 4-month-old female NOD/SCID.e2f1+/+ and NOD/SCID.e2f1−/− mice fed water (A) or 1% sucrose water (B) overnight were poured on YPD agar. Other samples in mice fed water (C) or 1% sucrose water (D) were poured on BHI agar. CFU data were obtained from three independent experiments with four mice from each strain, and values are expressed as the means ± standard deviations (SDs) of the data. Asterisks show significant differences (*P <0.05) in A and significant differences (** <0.05) between water (C) and 1% sucrose water (D) for drinking.