Germline intergenic duplications at Xq26.1 underlie Bazex-Dupré-Christol basal cell carcinoma susceptibility syndrome

Yanshan Liu; Siddharth Banka; Yingzhi Huang; Jonathan Hardman-Smart; Derek Pye; Antonio Torrelo; Glenda M Beaman; Marcelo G Kazanietz; Martin J Baker; Carlo Ferrazzano; Chenfu Shi; Gisela Orozco; Stephen Eyre; Michel van Geel; Anette Bygum; Judith Fischer; Zosia Miedzybrodzka; Faris Abuzahra; Albert Rübben; Sara Cuvertino; Jamie M Ellingford; Miriam J Smith; D Gareth Evans; Lizelotte J M T Weppner-Parren; Maurice A M van Steensel; Iskander H Chaudhary; D Chas Mangham; John T Lear; Ralf Paus; Jorge Frank; William G Newman; Xue Zhang

doi:10.1111/bjd.21842

Germline intergenic duplications at Xq26.1 underlie Bazex-Dupré-Christol basal cell carcinoma susceptibility syndrome

Yanshan Liu, Siddharth Banka, Yingzhi Huang, Jonathan Hardman-Smart, Derek Pye, Antonio Torrelo, Glenda M Beaman, Marcelo G Kazanietz, Martin J Baker, Carlo Ferrazzano, Chenfu Shi, Gisela Orozco, Stephen Eyre, Michel van Geel, Anette Bygum, Judith Fischer, Zosia Miedzybrodzka, Faris Abuzahra, Albert Rübben, Sara CuvertinoJamie M Ellingford, Miriam J Smith, D Gareth Evans, Lizelotte J M T Weppner-Parren, Maurice A M van Steensel, Iskander H Chaudhary, D Chas Mangham, John T Lear, Ralf Paus, Jorge Frank, William G Newman, Xue Zhang^* (Corresponding Author)

^*Corresponding author for this work

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Abstract

BACKGROUND: Bazex-Dupré-Christol syndrome (BDCS; MIM301845) is a rare X-linked dominant genodermatosis characterized by follicular atrophoderma, congenital hypotrichosis and multiple basal cell carcinomas (BCCs). Previous studies have linked BDCS to an 11·4-Mb interval on chromosome Xq25-q27.1. However, the genetic mechanism of BDCS remains an open question.

OBJECTIVES: To investigate the genetic aetiology and molecular mechanisms underlying BDCS.

METHODS: We ascertained multiple individuals from eight unrelated families affected with BDCS (F1-F8). Whole-exome (F1 and F2) and genome sequencing (F3) were performed to identify putative disease-causing variants within the linkage region. Array comparative genomic hybridization and quantitative polymerase chain reaction (PCR) were used to explore copy number variations, followed by long-range gap PCR and Sanger sequencing to amplify the duplication junctions and to define the head-tail junctions. Hi-C was performed on dermal fibroblasts from two affected individuals with BDCS and one control. Public datasets and tools were used to identify regulatory elements and transcription factor binding sites within the minimal duplicated region. Immunofluorescence was performed in hair follicles, BCCs and trichoepitheliomas from patients with BDCS and sporadic BCCs. The ACTRT1 variant c.547dup (p.Met183Asnfs*17), previously proposed to cause BDCS, was evaluated with t allele frequency calculator.

RESULTS: In eight families with BDCS, we identified overlapping 18-135-kb duplications (six inherited and two de novo) at Xq26.1, flanked by ARHGAP36 and IGSF1. Hi-C showed that the duplications did not affect the topologically associated domain, but may alter the interactions between flanking genes and putative enhancers located in the minimal duplicated region. We detected ARHGAP36 expression near the control hair follicular stem cell compartment, and found increased ARHGAP36 levels in hair follicles in telogen, in BCCs and in trichoepitheliomas from patients with BDCS. ARHGAP36 was also detected in sporadic BCCs from individuals without BDCS. Our modelling showed the predicted maximum tolerated minor allele frequency of ACTRT1 variants in control populations to be orders of magnitude higher than expected for a high-penetrant ultra-rare disorder, suggesting loss of function of ACTRT1 variants to be an unlikely cause for BDCS.

CONCLUSIONS: Noncoding Xq26.1 duplications cause BDCS. The BDCS duplications most likely lead to dysregulation of ARHGAP36. ARHGAP36 is a potential therapeutic target for both inherited and sporadic BCCs. What is already known about this topic? Bazex-Dupré-Christol syndrome (BDCS) is a rare X-linked basal cell carcinoma susceptibility syndrome linked to an 11·4-Mb interval on chromosome Xq25-q27.1. Loss-of-function variants in ACTRT1 and its regulatory elements were suggested to cause BDCS. What does this study add? BDCS is caused by small tandem noncoding intergenic duplications at chromosome Xq26.1. The Xq26.1 BDCS duplications likely dysregulate ARHGAP36, the flanking centromeric gene. ACTRT1 loss-of-function variants are unlikely to cause BDCS. What is the translational message? This study provides the basis for accurate genetic testing for BDCS, which will aid precise diagnosis and appropriate surveillance and clinical management. ARHGAP36 may be a novel therapeutic target for all forms of sporadic basal cell carcinomas.

Original language	English
Pages (from-to)	948-961
Number of pages	15
Journal	British Journal of Dermatology
Volume	187
Issue number	6
Early online date	12 Sept 2022
DOIs	https://doi.org/10.1111/bjd.21842
Publication status	Published - 4 Dec 2022

Bibliographical note

Funding sources
X.Z. is supported by the National Natural Science Foundation of China (grant number 81788101), the CAMS Innovation Fund for Medical Sciences (grant numbers 2021-I2M-1-018 and 2016-I2M-1-002) and the National Key Research and Development Program of China (grant number 2016YFC0905100). M.J.S., D.G.E., R.P. and W.G.N. are supported by the Manchester NIHR Biomedical Research Centre (IS-BRC-1215-20007). Z.M. is supported by the NHS Grampian Biorepository (NHS Scotland). J.M.E. is funded by a postdoctoral research fellowship from the Health Education England Genomics Education Programme. G.O. and C.S. are funded by Wellcome Trust awards (207491/Z/17/Z for G.O., 215207/Z/19/Z for C.S.). G.O., C.S. and S.E. are supported by a Versus Arthritis award (21754) and NIHR Manchester BRC. S.E. is supported by a Medical Research Council award (MR/N00017X/1).

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Liu, Y., Banka, S., Huang, Y., Hardman-Smart, J., Pye, D., Torrelo, A., Beaman, G. M., Kazanietz, M. G., Baker, M. J., Ferrazzano, C., Shi, C., Orozco, G., Eyre, S., van Geel, M., Bygum, A., Fischer, J., Miedzybrodzka, Z., Abuzahra, F., Rübben, A., ... Zhang, X. (2022). Germline intergenic duplications at Xq26.1 underlie Bazex-Dupré-Christol basal cell carcinoma susceptibility syndrome. British Journal of Dermatology, 187(6), 948-961. https://doi.org/10.1111/bjd.21842

Liu, Y, Banka, S, Huang, Y, Hardman-Smart, J, Pye, D, Torrelo, A, Beaman, GM, Kazanietz, MG, Baker, MJ, Ferrazzano, C, Shi, C, Orozco, G, Eyre, S, van Geel, M, Bygum, A, Fischer, J, Miedzybrodzka, Z, Abuzahra, F, Rübben, A, Cuvertino, S, Ellingford, JM, Smith, MJ, Evans, DG, Weppner-Parren, LJMT, van Steensel, MAM, Chaudhary, IH, Mangham, DC, Lear, JT, Paus, R, Frank, J, Newman, WG & Zhang, X 2022, 'Germline intergenic duplications at Xq26.1 underlie Bazex-Dupré-Christol basal cell carcinoma susceptibility syndrome', British Journal of Dermatology, vol. 187, no. 6, pp. 948-961. https://doi.org/10.1111/bjd.21842

@article{6951dfa1ceb248fda28825ec3cc0318e,

title = "Germline intergenic duplications at Xq26.1 underlie Bazex-Dupr{\'e}-Christol basal cell carcinoma susceptibility syndrome",

abstract = "BACKGROUND: Bazex-Dupr{\'e}-Christol syndrome (BDCS; MIM301845) is a rare X-linked dominant genodermatosis characterized by follicular atrophoderma, congenital hypotrichosis and multiple basal cell carcinomas (BCCs). Previous studies have linked BDCS to an 11·4-Mb interval on chromosome Xq25-q27.1. However, the genetic mechanism of BDCS remains an open question.OBJECTIVES: To investigate the genetic aetiology and molecular mechanisms underlying BDCS.METHODS: We ascertained multiple individuals from eight unrelated families affected with BDCS (F1-F8). Whole-exome (F1 and F2) and genome sequencing (F3) were performed to identify putative disease-causing variants within the linkage region. Array comparative genomic hybridization and quantitative polymerase chain reaction (PCR) were used to explore copy number variations, followed by long-range gap PCR and Sanger sequencing to amplify the duplication junctions and to define the head-tail junctions. Hi-C was performed on dermal fibroblasts from two affected individuals with BDCS and one control. Public datasets and tools were used to identify regulatory elements and transcription factor binding sites within the minimal duplicated region. Immunofluorescence was performed in hair follicles, BCCs and trichoepitheliomas from patients with BDCS and sporadic BCCs. The ACTRT1 variant c.547dup (p.Met183Asnfs*17), previously proposed to cause BDCS, was evaluated with t allele frequency calculator.RESULTS: In eight families with BDCS, we identified overlapping 18-135-kb duplications (six inherited and two de novo) at Xq26.1, flanked by ARHGAP36 and IGSF1. Hi-C showed that the duplications did not affect the topologically associated domain, but may alter the interactions between flanking genes and putative enhancers located in the minimal duplicated region. We detected ARHGAP36 expression near the control hair follicular stem cell compartment, and found increased ARHGAP36 levels in hair follicles in telogen, in BCCs and in trichoepitheliomas from patients with BDCS. ARHGAP36 was also detected in sporadic BCCs from individuals without BDCS. Our modelling showed the predicted maximum tolerated minor allele frequency of ACTRT1 variants in control populations to be orders of magnitude higher than expected for a high-penetrant ultra-rare disorder, suggesting loss of function of ACTRT1 variants to be an unlikely cause for BDCS.CONCLUSIONS: Noncoding Xq26.1 duplications cause BDCS. The BDCS duplications most likely lead to dysregulation of ARHGAP36. ARHGAP36 is a potential therapeutic target for both inherited and sporadic BCCs. What is already known about this topic? Bazex-Dupr{\'e}-Christol syndrome (BDCS) is a rare X-linked basal cell carcinoma susceptibility syndrome linked to an 11·4-Mb interval on chromosome Xq25-q27.1. Loss-of-function variants in ACTRT1 and its regulatory elements were suggested to cause BDCS. What does this study add? BDCS is caused by small tandem noncoding intergenic duplications at chromosome Xq26.1. The Xq26.1 BDCS duplications likely dysregulate ARHGAP36, the flanking centromeric gene. ACTRT1 loss-of-function variants are unlikely to cause BDCS. What is the translational message? This study provides the basis for accurate genetic testing for BDCS, which will aid precise diagnosis and appropriate surveillance and clinical management. ARHGAP36 may be a novel therapeutic target for all forms of sporadic basal cell carcinomas.",

author = "Yanshan Liu and Siddharth Banka and Yingzhi Huang and Jonathan Hardman-Smart and Derek Pye and Antonio Torrelo and Beaman, {Glenda M} and Kazanietz, {Marcelo G} and Baker, {Martin J} and Carlo Ferrazzano and Chenfu Shi and Gisela Orozco and Stephen Eyre and {van Geel}, Michel and Anette Bygum and Judith Fischer and Zosia Miedzybrodzka and Faris Abuzahra and Albert R{\"u}bben and Sara Cuvertino and Ellingford, {Jamie M} and Smith, {Miriam J} and Evans, {D Gareth} and Weppner-Parren, {Lizelotte J M T} and {van Steensel}, {Maurice A M} and Chaudhary, {Iskander H} and Mangham, {D Chas} and Lear, {John T} and Ralf Paus and Jorge Frank and Newman, {William G} and Xue Zhang",

note = "Funding sources X.Z. is supported by the National Natural Science Foundation of China (grant number 81788101), the CAMS Innovation Fund for Medical Sciences (grant numbers 2021-I2M-1-018 and 2016-I2M-1-002) and the National Key Research and Development Program of China (grant number 2016YFC0905100). M.J.S., D.G.E., R.P. and W.G.N. are supported by the Manchester NIHR Biomedical Research Centre (IS-BRC-1215-20007). Z.M. is supported by the NHS Grampian Biorepository (NHS Scotland). J.M.E. is funded by a postdoctoral research fellowship from the Health Education England Genomics Education Programme. G.O. and C.S. are funded by Wellcome Trust awards (207491/Z/17/Z for G.O., 215207/Z/19/Z for C.S.). G.O., C.S. and S.E. are supported by a Versus Arthritis award (21754) and NIHR Manchester BRC. S.E. is supported by a Medical Research Council award (MR/N00017X/1).",

year = "2022",

month = dec,

day = "4",

doi = "10.1111/bjd.21842",

language = "English",

volume = "187",

pages = "948--961",

journal = "British Journal of Dermatology",

issn = "0007-0963",

publisher = "Oxford University Press (OUP)",

number = "6",

}

TY - JOUR

T1 - Germline intergenic duplications at Xq26.1 underlie Bazex-Dupré-Christol basal cell carcinoma susceptibility syndrome

AU - Liu, Yanshan

AU - Banka, Siddharth

AU - Huang, Yingzhi

AU - Hardman-Smart, Jonathan

AU - Pye, Derek

AU - Torrelo, Antonio

AU - Beaman, Glenda M

AU - Kazanietz, Marcelo G

AU - Baker, Martin J

AU - Ferrazzano, Carlo

AU - Shi, Chenfu

AU - Orozco, Gisela

AU - Eyre, Stephen

AU - van Geel, Michel

AU - Bygum, Anette

AU - Fischer, Judith

AU - Miedzybrodzka, Zosia

AU - Abuzahra, Faris

AU - Rübben, Albert

AU - Cuvertino, Sara

AU - Ellingford, Jamie M

AU - Smith, Miriam J

AU - Evans, D Gareth

AU - Weppner-Parren, Lizelotte J M T

AU - van Steensel, Maurice A M

AU - Chaudhary, Iskander H

AU - Mangham, D Chas

AU - Lear, John T

AU - Paus, Ralf

AU - Frank, Jorge

AU - Newman, William G

AU - Zhang, Xue

N1 - Funding sources X.Z. is supported by the National Natural Science Foundation of China (grant number 81788101), the CAMS Innovation Fund for Medical Sciences (grant numbers 2021-I2M-1-018 and 2016-I2M-1-002) and the National Key Research and Development Program of China (grant number 2016YFC0905100). M.J.S., D.G.E., R.P. and W.G.N. are supported by the Manchester NIHR Biomedical Research Centre (IS-BRC-1215-20007). Z.M. is supported by the NHS Grampian Biorepository (NHS Scotland). J.M.E. is funded by a postdoctoral research fellowship from the Health Education England Genomics Education Programme. G.O. and C.S. are funded by Wellcome Trust awards (207491/Z/17/Z for G.O., 215207/Z/19/Z for C.S.). G.O., C.S. and S.E. are supported by a Versus Arthritis award (21754) and NIHR Manchester BRC. S.E. is supported by a Medical Research Council award (MR/N00017X/1).

PY - 2022/12/4

Y1 - 2022/12/4

N2 - BACKGROUND: Bazex-Dupré-Christol syndrome (BDCS; MIM301845) is a rare X-linked dominant genodermatosis characterized by follicular atrophoderma, congenital hypotrichosis and multiple basal cell carcinomas (BCCs). Previous studies have linked BDCS to an 11·4-Mb interval on chromosome Xq25-q27.1. However, the genetic mechanism of BDCS remains an open question.OBJECTIVES: To investigate the genetic aetiology and molecular mechanisms underlying BDCS.METHODS: We ascertained multiple individuals from eight unrelated families affected with BDCS (F1-F8). Whole-exome (F1 and F2) and genome sequencing (F3) were performed to identify putative disease-causing variants within the linkage region. Array comparative genomic hybridization and quantitative polymerase chain reaction (PCR) were used to explore copy number variations, followed by long-range gap PCR and Sanger sequencing to amplify the duplication junctions and to define the head-tail junctions. Hi-C was performed on dermal fibroblasts from two affected individuals with BDCS and one control. Public datasets and tools were used to identify regulatory elements and transcription factor binding sites within the minimal duplicated region. Immunofluorescence was performed in hair follicles, BCCs and trichoepitheliomas from patients with BDCS and sporadic BCCs. The ACTRT1 variant c.547dup (p.Met183Asnfs*17), previously proposed to cause BDCS, was evaluated with t allele frequency calculator.RESULTS: In eight families with BDCS, we identified overlapping 18-135-kb duplications (six inherited and two de novo) at Xq26.1, flanked by ARHGAP36 and IGSF1. Hi-C showed that the duplications did not affect the topologically associated domain, but may alter the interactions between flanking genes and putative enhancers located in the minimal duplicated region. We detected ARHGAP36 expression near the control hair follicular stem cell compartment, and found increased ARHGAP36 levels in hair follicles in telogen, in BCCs and in trichoepitheliomas from patients with BDCS. ARHGAP36 was also detected in sporadic BCCs from individuals without BDCS. Our modelling showed the predicted maximum tolerated minor allele frequency of ACTRT1 variants in control populations to be orders of magnitude higher than expected for a high-penetrant ultra-rare disorder, suggesting loss of function of ACTRT1 variants to be an unlikely cause for BDCS.CONCLUSIONS: Noncoding Xq26.1 duplications cause BDCS. The BDCS duplications most likely lead to dysregulation of ARHGAP36. ARHGAP36 is a potential therapeutic target for both inherited and sporadic BCCs. What is already known about this topic? Bazex-Dupré-Christol syndrome (BDCS) is a rare X-linked basal cell carcinoma susceptibility syndrome linked to an 11·4-Mb interval on chromosome Xq25-q27.1. Loss-of-function variants in ACTRT1 and its regulatory elements were suggested to cause BDCS. What does this study add? BDCS is caused by small tandem noncoding intergenic duplications at chromosome Xq26.1. The Xq26.1 BDCS duplications likely dysregulate ARHGAP36, the flanking centromeric gene. ACTRT1 loss-of-function variants are unlikely to cause BDCS. What is the translational message? This study provides the basis for accurate genetic testing for BDCS, which will aid precise diagnosis and appropriate surveillance and clinical management. ARHGAP36 may be a novel therapeutic target for all forms of sporadic basal cell carcinomas.

AB - BACKGROUND: Bazex-Dupré-Christol syndrome (BDCS; MIM301845) is a rare X-linked dominant genodermatosis characterized by follicular atrophoderma, congenital hypotrichosis and multiple basal cell carcinomas (BCCs). Previous studies have linked BDCS to an 11·4-Mb interval on chromosome Xq25-q27.1. However, the genetic mechanism of BDCS remains an open question.OBJECTIVES: To investigate the genetic aetiology and molecular mechanisms underlying BDCS.METHODS: We ascertained multiple individuals from eight unrelated families affected with BDCS (F1-F8). Whole-exome (F1 and F2) and genome sequencing (F3) were performed to identify putative disease-causing variants within the linkage region. Array comparative genomic hybridization and quantitative polymerase chain reaction (PCR) were used to explore copy number variations, followed by long-range gap PCR and Sanger sequencing to amplify the duplication junctions and to define the head-tail junctions. Hi-C was performed on dermal fibroblasts from two affected individuals with BDCS and one control. Public datasets and tools were used to identify regulatory elements and transcription factor binding sites within the minimal duplicated region. Immunofluorescence was performed in hair follicles, BCCs and trichoepitheliomas from patients with BDCS and sporadic BCCs. The ACTRT1 variant c.547dup (p.Met183Asnfs*17), previously proposed to cause BDCS, was evaluated with t allele frequency calculator.RESULTS: In eight families with BDCS, we identified overlapping 18-135-kb duplications (six inherited and two de novo) at Xq26.1, flanked by ARHGAP36 and IGSF1. Hi-C showed that the duplications did not affect the topologically associated domain, but may alter the interactions between flanking genes and putative enhancers located in the minimal duplicated region. We detected ARHGAP36 expression near the control hair follicular stem cell compartment, and found increased ARHGAP36 levels in hair follicles in telogen, in BCCs and in trichoepitheliomas from patients with BDCS. ARHGAP36 was also detected in sporadic BCCs from individuals without BDCS. Our modelling showed the predicted maximum tolerated minor allele frequency of ACTRT1 variants in control populations to be orders of magnitude higher than expected for a high-penetrant ultra-rare disorder, suggesting loss of function of ACTRT1 variants to be an unlikely cause for BDCS.CONCLUSIONS: Noncoding Xq26.1 duplications cause BDCS. The BDCS duplications most likely lead to dysregulation of ARHGAP36. ARHGAP36 is a potential therapeutic target for both inherited and sporadic BCCs. What is already known about this topic? Bazex-Dupré-Christol syndrome (BDCS) is a rare X-linked basal cell carcinoma susceptibility syndrome linked to an 11·4-Mb interval on chromosome Xq25-q27.1. Loss-of-function variants in ACTRT1 and its regulatory elements were suggested to cause BDCS. What does this study add? BDCS is caused by small tandem noncoding intergenic duplications at chromosome Xq26.1. The Xq26.1 BDCS duplications likely dysregulate ARHGAP36, the flanking centromeric gene. ACTRT1 loss-of-function variants are unlikely to cause BDCS. What is the translational message? This study provides the basis for accurate genetic testing for BDCS, which will aid precise diagnosis and appropriate surveillance and clinical management. ARHGAP36 may be a novel therapeutic target for all forms of sporadic basal cell carcinomas.

U2 - 10.1111/bjd.21842

DO - 10.1111/bjd.21842

M3 - Article

C2 - 35986704

SN - 0007-0963

VL - 187

SP - 948

EP - 961

JO - British Journal of Dermatology

JF - British Journal of Dermatology

IS - 6

ER -

Germline intergenic duplications at Xq26.1 underlie Bazex-Dupré-Christol basal cell carcinoma susceptibility syndrome

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