Clinically significant micafungin resistance in Candida albicans involves modification of a glucan synthase catalytic subunit GSC1 (FKS1) allele followed by loss of heterozygosity

K. Niimi; B. C. Monk; A. Hirai; K. Hatakenaka; T. Umeyama; E. Lamping; K. Maki; K. Tanabe; T. Kamimura; F. Ikeda; Y. Uehara; R. Kano; A. Hasegawa; R. D. Cannon; M. Niimi

doi:10.1093/jac/dkq073

Clinically significant micafungin resistance in Candida albicans involves modification of a glucan synthase catalytic subunit GSC1 (FKS1) allele followed by loss of heterozygosity

K. Niimi, B. C. Monk, A. Hirai, K. Hatakenaka, T. Umeyama, E. Lamping, K. Maki, K. Tanabe, T. Kamimura, F. Ikeda, Y. Uehara, R. Kano, A. Hasegawa, R. D. Cannon, M. Niimi

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49 Scopus citations

Abstract

Objectives: To determine the mechanism of intermediate-and high-level echinocandin resistance, resulting from heterozygous and homozygous mutations in GSC1 (FKS1), in both laboratory-generated and clinical isolates of Candida albicans. Methods: The DNA sequences of the entire open reading frames of GSC1, GSL1 (FKS3) and RHO1, which may contribute to the β-1,3-glucan synthase of a micafungin-susceptible strain and a resistant clinical isolate, were compared. A spontaneous heterozygous mutant isolated by selection for micafungin resistance, and a panel of laboratory-generated homozygous and heterozygous mutants that possessed combinations of the echinocandin-susceptible and -resistant alleles, or mutants with individual GSC1 alleles deleted, were used to compare levels of echinocandin resistance and inhibition of glucan synthase activity. Results: DNA sequence analysis identified a mutation, S645P, in both alleles of GSC1 from the clinical isolate. GSL1 had two homozygous amino acid changes and five non-synonymous nucleotide polymorphisms due to allelic variation. The predicted amino acid sequence of Rho1p was conserved between strains. Reconstruction of the heterozygous (S645/S645F) and homozygous (S645F/S645F) mutation showed that the homozygous mutation conferred a higher level of micafungin resistance (4 mg/L) than the heterozygous mutation (1 mg/L). Exposure of the heterozygous mutant to micafungin resulted in a loss of heterozygosity. Kinetic analysis of β-1,3-glucan synthase activity showed that the homozygous and heterozygous mutations gave echinocandin susceptibility profiles that correlated with their MIC values. Conclusions: A homozygous hot-spot mutation in GSC1, caused by mutation in one allele and then loss of heterozygosity, is required for high-level echinocandin resistance in C. albicans. Both alleles of GSC1 contribute equally and independently to β-1,3-glucan synthase activity.

Original language	English
Article number	dkq073
Pages (from-to)	842-852
Number of pages	11
Journal	Journal of Antimicrobial Chemotherapy
Volume	65
Issue number	5
DOIs	https://doi.org/10.1093/jac/dkq073
State	Published - 16 Mar 2010
Externally published	Yes

Keywords

C. albicans
Drug resistance
Echinocandins

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10.1093/jac/dkq073

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Niimi, K., Monk, B. C., Hirai, A., Hatakenaka, K., Umeyama, T., Lamping, E., Maki, K., Tanabe, K., Kamimura, T., Ikeda, F., Uehara, Y., Kano, R., Hasegawa, A., Cannon, R. D., & Niimi, M. (2010). Clinically significant micafungin resistance in Candida albicans involves modification of a glucan synthase catalytic subunit GSC1 (FKS1) allele followed by loss of heterozygosity. Journal of Antimicrobial Chemotherapy, 65(5), 842-852. Article dkq073. https://doi.org/10.1093/jac/dkq073

@article{615014e962f54abe8cb61c56a5363765,

title = "Clinically significant micafungin resistance in Candida albicans involves modification of a glucan synthase catalytic subunit GSC1 (FKS1) allele followed by loss of heterozygosity",

abstract = "Objectives: To determine the mechanism of intermediate-and high-level echinocandin resistance, resulting from heterozygous and homozygous mutations in GSC1 (FKS1), in both laboratory-generated and clinical isolates of Candida albicans. Methods: The DNA sequences of the entire open reading frames of GSC1, GSL1 (FKS3) and RHO1, which may contribute to the β-1,3-glucan synthase of a micafungin-susceptible strain and a resistant clinical isolate, were compared. A spontaneous heterozygous mutant isolated by selection for micafungin resistance, and a panel of laboratory-generated homozygous and heterozygous mutants that possessed combinations of the echinocandin-susceptible and -resistant alleles, or mutants with individual GSC1 alleles deleted, were used to compare levels of echinocandin resistance and inhibition of glucan synthase activity. Results: DNA sequence analysis identified a mutation, S645P, in both alleles of GSC1 from the clinical isolate. GSL1 had two homozygous amino acid changes and five non-synonymous nucleotide polymorphisms due to allelic variation. The predicted amino acid sequence of Rho1p was conserved between strains. Reconstruction of the heterozygous (S645/S645F) and homozygous (S645F/S645F) mutation showed that the homozygous mutation conferred a higher level of micafungin resistance (4 mg/L) than the heterozygous mutation (1 mg/L). Exposure of the heterozygous mutant to micafungin resulted in a loss of heterozygosity. Kinetic analysis of β-1,3-glucan synthase activity showed that the homozygous and heterozygous mutations gave echinocandin susceptibility profiles that correlated with their MIC values. Conclusions: A homozygous hot-spot mutation in GSC1, caused by mutation in one allele and then loss of heterozygosity, is required for high-level echinocandin resistance in C. albicans. Both alleles of GSC1 contribute equally and independently to β-1,3-glucan synthase activity.",

keywords = "C. albicans, Drug resistance, Echinocandins",

author = "K. Niimi and Monk, {B. C.} and A. Hirai and K. Hatakenaka and T. Umeyama and E. Lamping and K. Maki and K. Tanabe and T. Kamimura and F. Ikeda and Y. Uehara and R. Kano and A. Hasegawa and Cannon, {R. D.} and M. Niimi",

year = "2010",

month = mar,

day = "16",

doi = "10.1093/jac/dkq073",

language = "英語",

volume = "65",

pages = "842--852",

journal = "Journal of Antimicrobial Chemotherapy",

issn = "0305-7453",

publisher = "Oxford University Press",

number = "5",

}

Niimi, K, Monk, BC, Hirai, A, Hatakenaka, K, Umeyama, T, Lamping, E, Maki, K, Tanabe, K, Kamimura, T, Ikeda, F, Uehara, Y, Kano, R, Hasegawa, A, Cannon, RD & Niimi, M 2010, 'Clinically significant micafungin resistance in Candida albicans involves modification of a glucan synthase catalytic subunit GSC1 (FKS1) allele followed by loss of heterozygosity', Journal of Antimicrobial Chemotherapy, vol. 65, no. 5, dkq073, pp. 842-852. https://doi.org/10.1093/jac/dkq073

Clinically significant micafungin resistance in Candida albicans involves modification of a glucan synthase catalytic subunit GSC1 (FKS1) allele followed by loss of heterozygosity. / Niimi, K.; Monk, B. C.; Hirai, A. et al.
In: Journal of Antimicrobial Chemotherapy, Vol. 65, No. 5, dkq073, 16.03.2010, p. 842-852.

Research output: Contribution to journal › Article › peer-review

TY - JOUR

T1 - Clinically significant micafungin resistance in Candida albicans involves modification of a glucan synthase catalytic subunit GSC1 (FKS1) allele followed by loss of heterozygosity

AU - Niimi, K.

AU - Monk, B. C.

AU - Hirai, A.

AU - Hatakenaka, K.

AU - Umeyama, T.

AU - Lamping, E.

AU - Maki, K.

AU - Tanabe, K.

AU - Kamimura, T.

AU - Ikeda, F.

AU - Uehara, Y.

AU - Kano, R.

AU - Hasegawa, A.

AU - Cannon, R. D.

AU - Niimi, M.

PY - 2010/3/16

Y1 - 2010/3/16

N2 - Objectives: To determine the mechanism of intermediate-and high-level echinocandin resistance, resulting from heterozygous and homozygous mutations in GSC1 (FKS1), in both laboratory-generated and clinical isolates of Candida albicans. Methods: The DNA sequences of the entire open reading frames of GSC1, GSL1 (FKS3) and RHO1, which may contribute to the β-1,3-glucan synthase of a micafungin-susceptible strain and a resistant clinical isolate, were compared. A spontaneous heterozygous mutant isolated by selection for micafungin resistance, and a panel of laboratory-generated homozygous and heterozygous mutants that possessed combinations of the echinocandin-susceptible and -resistant alleles, or mutants with individual GSC1 alleles deleted, were used to compare levels of echinocandin resistance and inhibition of glucan synthase activity. Results: DNA sequence analysis identified a mutation, S645P, in both alleles of GSC1 from the clinical isolate. GSL1 had two homozygous amino acid changes and five non-synonymous nucleotide polymorphisms due to allelic variation. The predicted amino acid sequence of Rho1p was conserved between strains. Reconstruction of the heterozygous (S645/S645F) and homozygous (S645F/S645F) mutation showed that the homozygous mutation conferred a higher level of micafungin resistance (4 mg/L) than the heterozygous mutation (1 mg/L). Exposure of the heterozygous mutant to micafungin resulted in a loss of heterozygosity. Kinetic analysis of β-1,3-glucan synthase activity showed that the homozygous and heterozygous mutations gave echinocandin susceptibility profiles that correlated with their MIC values. Conclusions: A homozygous hot-spot mutation in GSC1, caused by mutation in one allele and then loss of heterozygosity, is required for high-level echinocandin resistance in C. albicans. Both alleles of GSC1 contribute equally and independently to β-1,3-glucan synthase activity.

AB - Objectives: To determine the mechanism of intermediate-and high-level echinocandin resistance, resulting from heterozygous and homozygous mutations in GSC1 (FKS1), in both laboratory-generated and clinical isolates of Candida albicans. Methods: The DNA sequences of the entire open reading frames of GSC1, GSL1 (FKS3) and RHO1, which may contribute to the β-1,3-glucan synthase of a micafungin-susceptible strain and a resistant clinical isolate, were compared. A spontaneous heterozygous mutant isolated by selection for micafungin resistance, and a panel of laboratory-generated homozygous and heterozygous mutants that possessed combinations of the echinocandin-susceptible and -resistant alleles, or mutants with individual GSC1 alleles deleted, were used to compare levels of echinocandin resistance and inhibition of glucan synthase activity. Results: DNA sequence analysis identified a mutation, S645P, in both alleles of GSC1 from the clinical isolate. GSL1 had two homozygous amino acid changes and five non-synonymous nucleotide polymorphisms due to allelic variation. The predicted amino acid sequence of Rho1p was conserved between strains. Reconstruction of the heterozygous (S645/S645F) and homozygous (S645F/S645F) mutation showed that the homozygous mutation conferred a higher level of micafungin resistance (4 mg/L) than the heterozygous mutation (1 mg/L). Exposure of the heterozygous mutant to micafungin resulted in a loss of heterozygosity. Kinetic analysis of β-1,3-glucan synthase activity showed that the homozygous and heterozygous mutations gave echinocandin susceptibility profiles that correlated with their MIC values. Conclusions: A homozygous hot-spot mutation in GSC1, caused by mutation in one allele and then loss of heterozygosity, is required for high-level echinocandin resistance in C. albicans. Both alleles of GSC1 contribute equally and independently to β-1,3-glucan synthase activity.

KW - C. albicans

KW - Drug resistance

KW - Echinocandins

UR - http://www.scopus.com/inward/record.url?scp=77953710273&partnerID=8YFLogxK

U2 - 10.1093/jac/dkq073

DO - 10.1093/jac/dkq073

M3 - 記事

C2 - 20233776

AN - SCOPUS:77953710273

SN - 0305-7453

VL - 65

SP - 842

EP - 852

JO - Journal of Antimicrobial Chemotherapy

JF - Journal of Antimicrobial Chemotherapy

IS - 5

M1 - dkq073

ER -

Clinically significant micafungin resistance in Candida albicans involves modification of a glucan synthase catalytic subunit GSC1 (FKS1) allele followed by loss of heterozygosity

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