Melanoma prone families with CDK4 germline mutation: phenotypic profile and associations with MC1R variants

Hanne Eknes Puntervoll; Xiaohong R Yang; Hildegunn Høberg Vetti; Ingeborg M Bachmann; Marie Françoise Avril; Meriem Benfodda; Caterina Catricalà; Stéphane Dalle; Anne B Duval-Modeste; Paola Ghiorzo; Paola Grammatico; Mark Harland; Nicholas K Hayward; Hui-Han Hu; Thomas Jouary; Tanguy Martin-Denavit; Aija Ozola; Jane M Palmer; Lorenza Pastorino; Dace Pjanova; Nadem Soufir; Solrun J Steine; Alexander J Stratigos; Luc Thomas; Julie Tinat; Hensin Tsao; Rūta Veinalde; Margaret A Tucker; Brigitte Bressac-de Paillerets; Julia A Newton-Bishop; Alisa M Goldstein; Lars A Akslen; Anders Molven

doi:10.1136/jmedgenet-2012-101455

. 2013 Feb 5;50(4):264–270. doi: 10.1136/jmedgenet-2012-101455

Melanoma prone families with CDK4 germline mutation: phenotypic profile and associations with MC1R variants

Hanne Eknes Puntervoll ¹, Xiaohong R Yang ², Hildegunn Høberg Vetti ³, Ingeborg M Bachmann ^1,⁴, Marie Françoise Avril ⁵, Meriem Benfodda ⁶, Caterina Catricalà ⁷, Stéphane Dalle ⁸, Anne B Duval-Modeste ⁹, Paola Ghiorzo ¹⁰, Paola Grammatico ¹¹, Mark Harland ¹², Nicholas K Hayward ¹³, Hui-Han Hu ⁶, Thomas Jouary ¹⁴, Tanguy Martin-Denavit ⁸, Aija Ozola ¹⁵, Jane M Palmer ¹³, Lorenza Pastorino ¹⁰, Dace Pjanova ¹⁵, Nadem Soufir ⁶, Solrun J Steine ¹, Alexander J Stratigos ¹⁶, Luc Thomas ⁸, Julie Tinat ¹⁷, Hensin Tsao ¹⁸, Rūta Veinalde ¹⁵, Margaret A Tucker ², Brigitte Bressac-de Paillerets ¹⁹, Julia A Newton-Bishop ¹², Alisa M Goldstein ², Lars A Akslen ^1,^20,²¹, Anders Molven ^1,²¹

¹Section for Pathology, The Gade Institute, University of Bergen, Bergen, Norway

²Division of Cancer Epidemiology and Genetics, National Cancer Institute, National Institutes of Health, Bethesda, Maryland, USA

³Western Norway Familial Cancer Center, Center for Medical Genetics and Molecular Medicine, Haukeland University Hospital, Bergen, Norway

⁴Department of Dermatology, Haukeland University Hospital, Bergen, Norway

⁵AP-HP, Hôpital Cochin-Tarnier, Université Paris Descartes, Paris, France

⁶AP-HP, Genetic Department, Bichat Hospital and INSERM U976, Cutaneous Research Center, Paris 7 University, Saint Louis Hospital, Paris, France

⁷Department of Dermatologic Oncology, San Gallicano Dermatologic Institute, IRCCS, Rome, Italy

⁸Unit of Dermatology, Université Claude Bernard Lyon 1, Centre Hospitalier Lyon-Sud, Hospices Civils de Lyon, Lyon, France

⁹Department of Dermatology, Rouen University Hospital, Rouen, France

¹⁰Department of Internal Medicine, University of Genoa and Laboratory of Genetics of Rare Hereditary Cancers, San Martino-IST Research Hospital, Genoa, Italy

¹¹Medical Genetics, Molecular Medicine Department, Sapienza University, S. Camillo-Forlanini Hospital, Rome, Italy

¹²Section of Epidemiology and Biostatistics, Leeds Institute of Molecular Medicine, Leeds Cancer Research UK Centre, St James's University Hospital, Leeds, UK

¹³Queensland Institute of Medical Research, Brisbane, Queensland, Australia

¹⁴Unité de Cancérologie Cutanée, Service de Dermatologie, Bordeaux, France

¹⁵Latvian Biomedical Research and Study Centre, Riga, Latvia

¹⁶Dermato-Oncology Unit, Department of Dermatology, University of Athens Medical School, Andreas Sygros Hospital, Athens, Greece

¹⁷Department of Genetics, Rouen University Hospital, Rouen, France

¹⁸Department of Dermatology, Wellman Center for Photomedicine, MGH Cancer Center, Massachusetts General Hospital, Boston, Massachusetts, USA

¹⁹Service de Génétique, Département de Biopathologie, Institut de Cancérologie Gustave Roussy, Villejuif and INSERM U946, Bâtiment IGM, Fondation Jean Dausset, Paris, France

²⁰Centre for Cancer Biomarkers, The Gade Institute, University of Bergen, Bergen, Norway

²¹Department of Pathology, Haukeland University Hospital, Bergen, Norway

^✉

Correspondence to Professor Anders Molven, Section for Pathology, The Gade Institute, University of Bergen, Haukeland University Hospital, N-5021 Bergen, Norway; anders.molven@gades.uib.no

PMCID: PMC3607098 PMID: 23384855

Abstract

Background

CDKN2A and CDK4 are high risk susceptibility genes for cutaneous malignant melanoma. Melanoma families with CDKN2A germline mutations have been extensively characterised, whereas CDK4 families are rare and lack a systematic investigation of their phenotype.

Methods

All known families with CDK4 germline mutations (n=17) were recruited for the study by contacting the authors of published papers or by requests via the Melanoma Genetics Consortium (GenoMEL). Phenotypic data related to primary melanoma and pigmentation characteristics were collected. The CDK4 exon 2 and the complete coding region of the MC1R gene were sequenced.

Results

Eleven families carried the CDK4 R24H mutation whereas six families had the R24C mutation. The total number of subjects with verified melanoma was 103, with a median age at first melanoma diagnosis of 39 years. Forty-three (41.7%) subjects had developed multiple primary melanomas (MPM). A CDK4 mutation was found in 89 (including 62 melanoma cases) of 209 tested subjects. CDK4 positive family members (both melanoma cases and unaffected subjects) were more likely to have clinically atypical nevi than CDK4 negative family members (p<0.001). MPM subjects had a higher frequency of MC1R red hair colour variants compared with subjects with one tumour (p=0.010).

Conclusion

Our study shows that families with CDK4 germline mutations cannot be distinguished phenotypically from CDKN2A melanoma families, which are characterised by early onset of disease, increased occurrence of clinically atypical nevi, and development of MPM. In a clinical setting, the CDK4 gene should therefore always be examined when a melanoma family tests negative for CDKN2A mutation.

Keywords: Molecular genetics, Cancer: dermatological, Genetic screening/counselling

Introduction

Cutaneous malignant melanoma is characterised by a complex aetiology, involving both genetic and environmental risk factors. Approximately 5–10% of the melanoma cases occur in a familial setting,¹ and two genes have so far been identified as high risk susceptibility genes for the disease: cyclin dependent kinase inhibitor 2A (CDKN2A)² ³ and cyclin dependent kinase 4 (CDK4).⁴ ⁵

CDKN2A (MIM 600160) encodes two distinct proteins, p16^INK4A and p14^ARF; both are tumour suppressors involved in cell cycle inhibition through different pathways.^6–8 In studies of melanoma families, the frequency of CDKN2A germline mutations is 20–40%, depending on the inclusion criteria.⁹ Common features of the CDKN2A melanoma families are early onset of disease and an increased risk of developing clinically atypical nevi, multiple primary melanomas (MPMs), and pancreatic cancer.¹⁰ ¹¹

CDK4 (MIM 123829) encodes the catalytic subunit of a heterodimeric Ser/Thr protein kinase, which together with its regulatory subunit (one of the D-type cyclins) is involved in controlling progression through the G1 phase of the cell cycle. Only 12 melanoma prone families with CDK4 germline mutations have been reported.⁴ ⁵ ^12–18 All mutations are located in codon 24 in exon 2, resulting in either an Arg24His (R24H) or Arg24Cys (R24C) substitution. This changes the p16^INK4A binding domain, leading to reduced p16^INK4A inhibition of CDK4 kinase activity and, subsequently, to cell cycle progression.¹⁹ ²⁰

Fair skin, red/blonde hair colour, freckling, and sun sensitivity are established pigmentation related risk factors for melanoma development. Pigmentation phenotype is partly regulated by the melanocortin-1 receptor (MC1R) gene (MIM 155555), a low risk melanoma susceptibility gene that may act both dependently and independently of ultraviolet radiation to influence melanoma risk.²¹ ²² MC1R encodes a seven-pass transmembrane, G-protein coupled receptor, which is involved in regulation of pheomelanin (yellow/red pigment) and eumelanin (black/brown pigment) production.²³ The MC1R locus is highly polymorphic in the Caucasian population,²⁴ and certain variants have been associated with the red hair colour (RHC) phenotype; that is, red hair, fair skin, freckling, and the inability to tan.²⁵ ²⁶ It is mainly the RHC variants that have been associated with increased melanoma risk,^27–29 although a link between non-RHC (NRHC) variants and melanoma has also been observed.³⁰ Studies within CDKN2A melanoma families have established that common MC1R variants act as modifier genes, in that carrying multiple variants is associated with increased melanoma risk. Several of these studies also reported an association between MC1R variants and decreased age at melanoma diagnosis, particularly in MPM patients.^31–35

A systematic characterisation of melanoma prone families with CDK4 germline mutation has never been performed. Previous studies of such families have included a limited number of melanoma cases and have mainly served to confirm CDK4 as a high risk melanoma gene. Here, we report a joint investigation of all 12 published CDK4 melanoma families along with five unpublished pedigrees. The purpose was to examine the clinical phenotype of these families, including possible modifying effects of MC1R variants, with the intent to inform genetic counselling internationally.

Methods

Recruitment of CDK4 mutated melanoma families and data collection

Melanoma families with germline CDK4 mutations were recruited for this study either by contacting the authors of published papers⁴ ⁵ ^12–18 or by requests for unpublished families via GenoMEL, the Melanoma Genetics Consortium (www.genomel.org). Seventeen families, including five unpublished, were enrolled (table 1).

Table 1.

Overview of the studied melanoma families with CDK4 germline mutations

Family designation	Laboratory number of family	Mutation	Subjects with verified cutaneous melanoma in pedigree	Total number of subjects with analysed DNA	Mutation positive family members	Mutation negative family members	Spouses	Reference
Norway-1	–	Arg24His	28	108	33	48	27	5
USA-1	8302	Arg24Cys	9	29	12	10	7	4
USA-2	8290	Arg24Cys	6	12	7	5	0	4
UK-1	301	Arg24His	4	5	2	2	1	5
UK-2	1119	Arg24Cys	5	7	4	3	0	Unpublished
Latvia-1	247	Arg24His	5	5	2	3	0	13
Latvia-2	268	Arg24His	5	6	3	3	0	16
Latvia-3	M679	Arg24His	5	3	2	0	1	Unpublished
Australia-1	60007	Arg24His	10	3	2	0	1	5
Italy-1	FM029	Arg24His	4	6	4	1	1	15
Italy-2	501153	Arg24Cys	1	2	1	1	0	18
France-1	759	Arg24His	6	14	9	3	2	12
France-2	–	Arg24His	2	4	3	0	1	14
France-3	–	Arg24Cys	2	1	1	0	0	Unpublished
France-4	14648	Arg24Cys	3	1	1	0	0	Unpublished
France-5	–	Arg24His	2	1	1	0	0	Unpublished
Greece-1	–	Arg24His	6	2	2	0	0	17
Total			103	209	89*	79	41

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*Sixty-two of the mutation positive family members had melanoma and 27 were unaffected.

Clinical examinations were performed by dermatologists or specifically trained research nurses, and phenotypic data were collected via a standardised form. Examiners were generally unaware of the genotype of individuals before recording clinical features. Data collected included skin type using the ‘Fitzpatrick classification’,³⁶ eye and hair colour, and total number of nevi (>2 mm in diameter). Also the presence of clinically atypical nevi, defined as nevi >5 mm with irregular pigmentation and an irregular or diffuse border,³⁷ was recorded. Diagnoses of cutaneous melanoma were confirmed by histology reports and/or medical records. For patients with MPMs, the total number of melanomas was recorded; however, age at melanoma diagnosis, anatomic location, and histological type were recorded only for the first three primaries. Anatomic location of the melanomas was categorised into head/neck, limbs, and trunk. Histologic type was recorded as superficial spreading melanoma (SSM), nodular melanoma (NM), lentigo malignant melanoma (LMM), in situ melanoma, and melanoma unclassified/classification unknown. No acral or mucosal melanomas were observed in our material. Information on non-melanoma cancers was collected for the melanoma cases and for those unaffected subjects who either had tested positive for a CDK4 mutation or were considered as obligate mutation carriers.

Written informed consent was obtained from the family members before enrolment. The study was performed according to the Helsinki declaration.

DNA analysis of CDK4 and MC1R

DNA samples were available from 209 subjects. Altogether, DNA from 62 melanoma cases, 106 unaffected family members (melanoma status not given for three of these; they were considered as unaffected in this study), and 41 spouses were examined for mutations in CDK4 exon 2 and for variants in the coding region of MC1R. The initial DNA analysis was performed by each individual research group, either by direct Sanger sequencing or by single strand conformation polymorphism screening; hence there was slight variation in protocols and primers.⁴ ⁵ ^12–18

Statistical analysis

Before the statistical analyses, hair and skin colour was grouped because of small sample sizes for these categorical variables: RHC versus all other hair colours, very fair/fair skin colour versus all other skin colours. For comparisons between subject groups (melanoma affected and unaffected CDK4 positive family members versus CDK4 negative family members and spouses) and different categorical variables (occurrence of clinically atypical nevi, melanoma status, hair and skin colour, MC1R variant distribution), the Pearson χ² test or the Fisher exact test were used depending on sample sizes. The non-parametric Mann–Whitney or Kruskal–Wallis tests were used to compare the continuous variable (age at first diagnosis) with the categorical variables (melanoma status, tumour location, histologic type, occurrence of clinically atypical nevi, MC1R variant distribution).

All observed MC1R variants were recorded, but because many variants were rare, they were grouped before the statistical comparisons with phenotypic data. These comparisons were performed as follows: (1) The distribution of individuals with MC1R consensus sequence, one and two MC1R variants was compared between the different subject groups (analysis denoted ‘Number of MC1R variants’). (2) The distribution of individuals with MC1R consensus sequence, RHC, NRHC, and RHC+NRHC variants was compared between the different subject groups (analysis denoted ‘Type of MC1R variants’). We observed no individuals with more than two MC1R variants. The RHC variants were defined as D84E, R142H, R151C, R160W, and D294H, all associated with red hair phenotype.²⁵ ²⁶ Other non-synonymous MC1R variants were labelled as NRHC. Synonymous MC1R variants were excluded from all analyses. When analysing MC1R variant distributions, the CDK4 negative family members and spouses were combined into a single control group.

Unconditional logistic regression analysis was used to assess whether atypical nevi status varied by melanoma affection and CDK4 carrier status when adjusted for age (age at last examination for unaffected subjects and age at diagnosis for melanoma patients). Statistical analyses were performed using the IBM Statistical Package for the Social Sciences, version 19 (SPSS Inc, Chicago, Illinois, USA) and SAS software (version 9.1.3, SAS Institute Inc, Cary, North Carolina, USA). p values<0.05 were considered to represent significant associations. Also p values between 0.05 and 0.10 are shown in the tables.

Results

Seventeen familial melanoma pedigrees with CDK4 germline mutations (11 with the R24H mutation and six with R24C) were available for this study; 12 previously published and five unpublished (table 1). In these pedigrees, a total of 103 members with cutaneous malignant melanoma (=affected subjects) were recorded. DNA was available for 209 subjects of whom 89 were mutation carriers (62 affected, 27 unaffected), 79 were mutation negative unaffected family members, and the remaining were spouses (table 1). As expected, all spouses had a normal CDK4 exon 2 sequence. Among the 41 affected subjects for whom DNA was not available, seven were classified as obligate mutation carriers. Of unaffected subjects without available DNA, five were obligate mutation carriers.

Phenotypic characteristics of melanoma patients in CDK4 families

Phenotypic characteristics of the 103 malignant melanoma cases are presented in table 2. Age at first malignant melanoma diagnosis was available for 95 cases and ranged from 18–86 years, with a median age of 39 years. Most cases occurred in the fourth decade of life (31.6%), whereas age of onset above age 60 years was rare (7.4%). There was no statistically significant difference in distribution of age at first diagnosis between males and females, or between cases with and without available DNA.

Table 2.

Phenotypic and genotypic characteristics of melanoma cases in families with CDK4 germline mutations

Variable*	Number	%
Sex (N=103)
Male	44	42.7
Female	59	57.3
Number of primary melanomas in affected subjects (N=103)
One	60	58.3
Multiple	43	41.7
Mean	2.1	–
CDK4 mutation status of affected subjects (N=103)
Subjects (N=77) in R24H families
CDK4 mutation positive	41	39.8
CDK4 mutation negative	0	0.0
Obligate CDK4 mutation carriers†	7	6.8
Unknown mutation status†	29	28.2
Subjects (N=26) in R24C families
CDK4 mutation positive	21	20.4
CDK4 mutation negative	0	0.0
Obligate CDK4 mutation carriers†	0	0.0
Unknown mutation status†	5	4.9
Age at first melanoma diagnosis (N=95)
<30 years	20	21.1
30–39 years	30	31.6
40–49 years	24	25.3
50–59 years	14	14.7
≥60 years	7	7.4
Missing data‡	8	–
Mean (years)	40.4	–
Median (years)	39.0	–
Anatomic location (N=140)§
Head/neck	31	22.1
Limbs	66	47.1
Trunk	43	30.7
Missing data‡	28	–
Anatomic location, first primary melanoma only (N=81)
Head/neck	17	21.0
Limbs	34	42.0
Trunk	30	37.0
Missing data‡	21	–
Histologic type (N=95)§
SSM	71	74.7
NM	3	3.2
LMM	1	1.1
In situ melanoma	20	21.1
Melanoma unclassified or classification unknown‡	73	–
Histologic type, first primary melanoma only (N=48)
SSM	34	70.8
NM	3	6.3
LMM	1	2.1
In situ melanoma	10	20.8
Melanoma unclassified or classification unknown‡	54	–

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*One melanoma case was recorded as MPM, but with no information on the actual number of melanomas. It was therefore excluded when calculating the mean number of melanomas and when summarising anatomic location and histologic type.

†DNA was not available for these cases.

‡Missing data are not included in the parentheses (N=) and not included when calculating percentages.

§For persons with MPM, information about the first three registered tumours was recorded.

LMM, lentigo malignant melanoma; MPM, multiple primary melanomas; NM, nodular melanoma; SSM, superficial spreading melanoma.

Forty-three melanoma patients (41.7%) developed more than one primary tumour. The number of primaries ranged from 2–13. Altogether, 217 melanomas were reported for 102 affected subjects (data on the number of melanomas were missing for one subject with MPM). Patients with MPMs showed a significantly lower median age at first diagnosis than patients with single primary melanoma (SPM): 35 and 43 years, respectively (p=0.002). There was no difference in distribution of SPM and MPM by gender.

The melanomas occurred most frequently on the limbs (table 2), and subjects with their first melanoma on this location had a significantly lower age at first diagnosis (33.5 years) than subjects with melanomas located in the head and neck region (45.5 years) (p=0.018). The predominant histologic type was SSM (table 2). Subjects with SSM had a significantly lower median age at first diagnosis than individuals with NM and LMM (p=0.039). The median ages were 36.5, 54, and 64 years, respectively. Ten of the first melanomas were recorded as in situ cases with a median diagnosis age of 33 years.

We further evaluated the occurrence of clinically atypical nevi (table 3). Both affected and unaffected CDK4 positive subjects showed a significantly higher frequency of atypical nevi (70% and 75%) than the CDK4 negative subjects (26.5%) (p<0.001). The associations remained significant after age adjustment (affected CDK4 positive patients: OR 6.08, 95% CI 2.51 to 14.76, p<0.001; unaffected CDK4 positive subjects: OR 7.37, 95% CI 1.99 to 27.39, p=0.003). The median age at first melanoma diagnosis for the atypical nevi positive patients was significantly lower (32.5 years) than for atypical nevi negative patients (40 years) (p=0.004).

Table 3.

Occurrence of clinically atypical nevi in families with CDK4 germline mutations

		CDK4 positive family members
	CDK4 negative family members	Affected		Unaffected
Clinically atypical nevi*	N=49 (%)	N=50 (%)	p Value†	N=20 (%)	p Value†
Present	13 (26.5)	35 (70.0)	<0.001	15 (75.0)	<0.001
Not present	36 (73.5)	15 (30.0)		5 (25.0)

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*Data on CDK4 mutation status and clinically atypical nevi were available for 119 subjects.

†CDK4 negative family members were compared with affected and with unaffected CDK4 positive family members, respectively.

There was no difference in distribution of hair and skin colour between the affected and unaffected CDK4 positive family members and the CDK4 negative family members (see online supplementary table 1). We also tested for phenotypic differences between subjects carrying the R24H and R24C mutations. No statistically significant differences were seen with regard to age at first melanoma diagnosis or the occurrence of MPM and clinically atypical nevi (see online supplementary table 2).

Concerning non-melanoma cancers, 33 cases were found in 25 of the 105 subjects where information on other cancers had been specified (see online supplementary table 3). Non-melanoma skin cancers and female related cancers were most frequently observed. Two cases of pancreatic cancer were seen. Ages of onset of the non-melanoma cancers were in a range expected in normal populations.

MC1R variants

Altogether, 15 different MC1R variants were observed in our material. Eleven variants predicted non-synonymous amino acid changes (V60L, V60R, D84E, V92M, R142H, R142S, R151C, I155T, R160W, R163Q, D294H), three variants corresponded to synonymous amino acid changes (A166A, Q233Q, T314T), and one was an insertion at the nucleotide level (86insA). V60R and R142S have, to our knowledge, not been reported before. R160W, R151C, and V60L were the most frequently observed variants. Five RHC variants were recorded: D84E, R142H, R151C, R160W, D294H. We classified all remaining non-synonymous MC1R variants and 86insA to the NRHC group.

There were no significant differences in MC1R variant distribution between the CDK4 negative family members and spouses. A control group was therefore established consisting of all CDK4 negative subjects. Comparison of the affected CDK4 mutation carriers with the CDK4 negative control group revealed no significant differences in the MC1R variant distribution (table 4). However, when comparing the unaffected CDK4 mutation carriers with the CDK4 negative control group, the former group showed a lower number of RHC variants (p=0.012). The unaffected CDK4 mutation carriers also had a significantly lower number of RHC variants compared with the affected CDK4 carriers (p=0.042) (table 4).

Table 4.

Frequencies of MC1R variants in families with CDK4 germline mutations

	CDK4 negative family members and spouses*	CDK4 positive family members†					Number of primary melanomas‡
		Unaffected		Affected			SPM	MPM
MC1R variant distribution	N=115 (%)	N=23 (%)	p Value§	N=60 (%)	p Value§	p Value¶	N=30 (%)	N=30 (%)	p Value**
Number of MC1R variants
0 (consensus sequence)	23 (20.0)	10 (43.5)	0.071	15 (25.0)	NS	NS	11 (36.7)	4 (13.3)	0.070
1 variant	71 (61.7)	10 (43.5)		32 (53.3)			15 (50.0)	17 (56.7)
2 variants	21 (18.3)	3 (13.0)		13 (21.7)			4 (13.3)	9 (30.0)
Type of MC1R variants
0 (consensus sequence)	23 (20.0)	10 (43.5)	0.012	15 (25.0)	NS	0.042	11 (36.7)	4 (13.3)	0.010
RHC only	48 (41.7)	3 (13.0)		23 (38.3)			7 (23.3)	16 (53.3)
NRHC only	31 (27.0)	9 (39.1)		14 (23.3)			10 (33.3)	4 (13.3)
Both RHC and NRHC	13 (11.3)	1 (4.4)		8 (13.3)			2 (6.7)	6 (20.0)

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*MC1R data were available for 76 of 79 CDK4 negative family members and for 39 of 41 spouses. In these groups, the distributions of number and type of MC1R variants were very similar, and the two groups were combined into a single control group for the statistical analyses.

†Melanoma status and MC1R data were available for 83 of 89 CDK4 positive family members.

‡The number of primary melanomas and MC1R data were available for 60 of the 103 melanoma subjects.

§The control group was compared with unaffected and affected CDK4 positive family members, respectively.

¶Unaffected mutation carriers were compared with affected mutation carriers.

**Subjects with SPM and MPM were compared with each other with regard to MC1R variant distribution.

NS=non-significant p value.

MPM, multiple primary melanomas; NRHC, non-red hair colour; RHC, red hair colour; SPM, single primary melanoma.

Finally, we investigated the MC1R variant distribution in MPM and SPM subjects (table 4). We found no statistically significant difference in the number of MC1R variants, but the MPM subjects were more likely to carry RHC variants (p=0.010). There were no significant associations between age at first melanoma diagnosis and MC1R variant distribution (tested in SPM and MPM subjects, both separately and combined). Similarly, there were no significant differences in the MC1R variant distribution in subjects with and without clinically atypical nevi.

Discussion

This study presents the largest dataset on melanoma families with CDK4 germline mutations to date, and is the first systematic evaluation of their phenotype and the influence of MC1R variants. We examined 17 families from eight countries that included 103 subjects with a verified melanoma diagnosis. The families carried either an R24H or R24C mutation, and we were not able to reveal any clinical differences between carriers of the two CDK4 mutations.

Early onset of disease is a characteristic feature of hereditary cancers. In this study, median age at first melanoma diagnosis was 39 years, about 15 years earlier than in the general Caucasian population. Thus, 21.1% of the melanoma patients in the CDK4 families had been diagnosed before the age of 30 years, whereas only 7.4% were diagnosed at age 60 years or older. Based on all individuals for which clinical information was available at age 50 years (or later), the mutation penetrance at this age was 74.2%. This confirms CDK4 as a highly penetrant melanoma risk gene. However, since most of the younger mutation carriers are now enrolled in screening programmes where severely dysplastic or borderline lesions are removed, the true lifetime melanoma risk of carrying a CDK4 germline mutation might be difficult to assess, assuming that such lesions are precursors.

We found that 41.7% of the melanoma subjects developed more than one primary melanoma, a frequency comparable to that observed in families with CDKN2A mutations.¹¹ ³⁸ ³⁹ Regarding clinically atypical nevi, a significantly higher occurrence was observed in the CDK4 mutation carriers compared with the CDK4 negative family members (table 3). Again, this is similar to findings in CDKN2A families.⁴⁰ ⁴¹ The presence of clinically atypical nevi has been suggested to be a modifier of melanoma risk in CDKN2A mutation carriers,⁴⁰ ⁴¹ and we observed that among affected subjects, the median age at first melanoma diagnosis was 7.5 years lower in atypical nevi positive than in negative family members. On the other hand, the frequency of these nevi was similar in affected and unaffected CDK4 positive subjects (table 3).

Unfortunately, a high number of the melanoma cases were unclassified with regard to histology, or classification could not be obtained from the patients’ records. This mainly concerned the oldest cases, as histology data generally became more complete for more recent cases. Nevertheless, the most frequent histologic type was SSM (74.7%), as in CDKN2A families.³⁹ The relatively high frequency of in situ melanomas (21.1%) may be influenced by increased surveillance of melanoma prone families.

We tried to assess non-melanoma cancers in our material, but encountered some obstacles. Firstly, most participating laboratories had collected anamnestic cancer data only from melanoma cases and CDK4 positive family members, and not from CDK4 negative members or spouses. Secondly, the CDK4 families stemmed from many countries and populations, with varying background incidences and different national registration systems for cancer. Thus, we were prevented from performing formal analyses to test whether the observed incidences of non-melanoma cancers (see online supplementary table 3) were higher than expected. Still, the frequencies of breast cancer and non-melanoma skin cancer might suggest that CDK4 mutation carriers could be at an increased risk. Sun exposure is an environmental determinant of risk for all skin cancers and an overrepresentation of non-melanoma skin cancer would therefore not be surprising. However, for all observed non-melanoma cancers, the median age of onset was similar to that of sporadic cases, so our data should be interpreted with caution.

When investigating the MC1R variant distribution, we observed that unaffected, CDK4 positive family members had a disproportionally low frequency of RHC variants, suggesting a biological influence. This difference may, however, be related to the smaller number of subjects in the unaffected, CDK4 positive group. Additionally, these subjects were generally younger (median age 28 years at last examination) than their affected relatives. It is therefore likely that some of the unaffected, CDK4 positive subjects eventually develop melanoma.

Looking at melanoma cases only, we found that the MPM subjects had a higher frequency of RHC type variants than the SPM subjects (table 4). Moreover, although not reaching statistical significance, MPM subjects also had the highest frequency of any MC1R variant (86.7% compared with 63.3% in SPM). These findings are consistent with previous observations in CDKN2A melanoma families.¹¹ ³⁸ ³⁹ We did not find any modifying effects of MC1R variants upon age at disease onset in the CDK4 families, in contrast to what has been reported for CDKN2A.^31–35

The current study has some limitations. Collection of data and biological material was performed by various groups in several different countries, and the data diverged in completeness. Small sample size due to lack of complete data contributes to low power in some statistical analyses and prohibited us from evaluating each MC1R variant separately. Despite these limitations, our study provides results informative for the clinical evaluation of CDK4 pedigrees.

Melanoma families with CDK4 germline mutations are very uncommon. However, codon 24 of this gene is likely to be a mutational hotspot and CDK4 families have been found in various countries, with several independent origins suggested by haplotype analysis.⁵ ¹³ ¹⁵ Our study suggests that CDK4 melanoma families are phenotypically similar to the CDKN2A families with regard to age of melanoma diagnosis, tumour localisation, histological type, and increased incidence of MPM and clinically atypical nevi. A general influence of MC1R variants on melanoma risk is seen in both types of melanoma families, although there may be some differences. We therefore conclude that it is not possible to distinguish CDK4 melanoma families from those with CDKN2A mutation based on the phenotype. The clinical implication is that, although CDK4 mutation carriers are rarely seen, exon 2 of this gene should be examined in melanoma families seeking gene testing whenever tests are negative for CDKN2A.

Supplementary Material

Web tables

jmedgenet-2012-101455-s1.pdf^{(100.1KB, pdf)}

Acknowledgments

This article is dedicated to the memory of Dr Magne B Grimstvedt (1925–2009), who in 1967 initiated studies on the large Norwegian melanoma family included here. Moreover, the authors are indebted to all participating family members, whose generosity and cooperation have made this study possible. We are also very grateful to the staff at the participating institutions for their contribution with regard to patient care and information for the data collection forms.

Footnotes

Contributors: HEP performed genotyping, collected all data from the participating research groups, tabulated the results, carried out the statistical analyses, and wrote the first manuscript draft. XRY and AMG provided data on the American families, and participated in the interpretation of data and statistical analyses. SJS, HHV, and IMB carried out genotyping, performed genetic counselling or dermatological examinations, and provided and interpreted clinical data for the Norwegian family. MAT, MH, JAN-B, AO, DP, RV, NKH, JMP, PGr, CC, PGh, LP, MFA, BBdeP, MB, H-HH, NS, TJ, ABD-M, JT, SD, TM-D, LT, AJS, and HT carried out genotyping, performed genetic counselling and dermatological examinations, and provided and interpreted clinical data for all other families included in the study. AM managed and designed the study in collaboration with AMG and LAA. The writing group consisted of HEP, XRY, AMG, LAA, and AM. All other authors have read and commented on the manuscript, and approved the final version.

Funding: The GenoMEL study was funded by the European Commission under the 6th Framework Programme (contract no. LSHC-CT-2006-018702), by Cancer Research UK Programme Awards (C588/A4994 and C588/A10589), by a Cancer Research UK Project grant (C8216/A6129), and by a grant from the US National Institutes of Health (NIH; CA83115). This research was also supported by a PhD fellowship from the University of Bergen to HEP, an INSERM Research Fellowship for hospital based scientists and an INCA coordinator or grant to BB-de P, and grants from the following sources: Norwegian Cancer Society (71512-PR-2006–0356); Intramural Research Program of the NIH, National Cancer Institute, Division of Cancer Epidemiology and Genetics; Leeds Cancer Research UK Centre (C37059/A11941); Latvian Council of Science (No. 10.0010.8); National Health and Medical Research Council of Australia; Italian Ministry of Health; PRIN 2008; Sapienza University of Rome; Institut National du Cancer PHRC 2007 (AOM 07, 195, N107004); Lyon 1 University; Hospices Civils de Lyon; Ligue Contre le Cancer du Rhone; and NIH (K24 CA149202).

Competing interests: None.

Patient consent: Obtained.

Ethics approval: Regional Ethics Committee REK-VEST, Norway (136.04).

Provenance and peer review: Not commissioned; externally peer reviewed.

Open Access: This is an Open Access article distributed in accordance with the Creative Commons Attribution Non Commercial (CC BY-NC 3.0) license, which permits others to distribute, remix, adapt, build upon this work non-commercially, and license their derivative works on different terms, provided the original work is properly cited and the use is non-commercial. See: http://creativecommons.org/licenses/by-nc/3.0/

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Associated Data

This section collects any data citations, data availability statements, or supplementary materials included in this article.

Supplementary Materials

Web tables

jmedgenet-2012-101455-s1.pdf^{(100.1KB, pdf)}

[R1] 1.Florell SR, Boucher KM, Garibotti G, Astle J, Kerber R, Mineau G, Wiggins C, Noyes RD, Tsodikov A, Cannon-Albright LA, Zone JJ, Samlowski WE, Leachman SA. Population-based analysis of prognostic factors and survival in familial melanoma. J Clin Oncol 2005;23:7168–77 [DOI] [PubMed] [Google Scholar]

[R2] 2.Hussussian CJ, Struewing JP, Goldstein AM, Higgins PA, Ally DS, Sheahan MD, Clark WH, Jr., Tucker MA, Dracopoli NC. Germline p16 mutations in familial melanoma. Nat Genet 1994;8:15–21 [DOI] [PubMed] [Google Scholar]

[R3] 3.Kamb A, Shattuck-Eidens D, Eeles R, Liu Q, Gruis NA, Ding W, Hussey C, Tran T, Miki Y, Weaver-Feldhaus J, McClure M, Aitken JF, Anderson DE, Bergman W, Frants R, Goldgar DE, Green A, MacLennan R, Martin NG, Meyer LJ, Youl P, Zone JJ, Skolnick MH, Cannon-Albright LA. Analysis of the p16 gene (CDKN2) as a candidate for the chromosome 9p melanoma susceptibility locus. Nat Genet 1994;8:23–6 [DOI] [PubMed] [Google Scholar]

[R4] 4.Zuo L, Weger J, Yang Q, Goldstein AM, Tucker MA, Walker GJ, Hayward N, Dracopoli NC. Germline mutations in the p16INK4a binding domain of CDK4 in familial melanoma. Nat Genet 1996;12:97–9 [DOI] [PubMed] [Google Scholar]

[R5] 5.Molven A, Grimstvedt MB, Steine SJ, Harland M, Avril MF, Hayward NK, Akslen LA. A large Norwegian family with inherited malignant melanoma, multiple atypical nevi, and CDK4 mutation. Genes Chromosomes Cancer 2005;44:10–8 [DOI] [PubMed] [Google Scholar]

[R6] 6.Serrano M, Hannon GJ, Beach D. A new regulatory motif in cell-cycle control causing specific inhibition of cyclin D/CDK4. Nature 1993;366:704–7 [DOI] [PubMed] [Google Scholar]

[R7] 7.Serrano M, Gomez-Lahoz E, DePinho RA, Beach D, Bar-Sagi D. Inhibition of ras-induced proliferation and cellular transformation by p16INK4. Science 1995;267:249–52 [DOI] [PubMed] [Google Scholar]

[R8] 8.Pomerantz J, Schreiber-Agus N, Liegeois NJ, Silverman A, Alland L, Chin L, Potes J, Chen K, Orlow I, Lee HW, Cordon-Cardo C, DePinho RA. The Ink4a tumor suppressor gene product, p19Arf, interacts with MDM2 and neutralizes MDM2's inhibition of p53. Cell 1998;92:713–23 [DOI] [PubMed] [Google Scholar]

[R9] 9.Goldstein AM, Chan M, Harland M, Gillanders EM, Hayward NK, Avril MF, Azizi E, Bianchi-Scarra G, Bishop DT, Bressac-de Paillerets B, Bruno W, Calista D, Albright LA Cannon, Demenais F, Elder DE, Ghiorzo P, Gruis NA, Hansson J, Hogg D, Holland EA, Kanetsky PA, Kefford RF, Landi MT, Lang J, Leachman SA, Mackie RM, Magnusson V, Mann GJ, Niendorf K, Bishop J Newton, Palmer JM, Puig S, Puig-Butille JA, de Snoo FA, Stark M, Tsao H, Tucker MA, Whitaker L, Yakobson E. High-risk melanoma susceptibility genes and pancreatic cancer, neural system tumors, and uveal melanoma across GenoMEL. Cancer Res 2006;66:9818–28 [DOI] [PubMed] [Google Scholar]

[R10] 10.Goldstein AM, Fraser MC, Struewing JP, Hussussian CJ, Ranade K, Zametkin DP, Fontaine LS, Organic SM, Dracopoli NC, Clark WH, Jr., Tucker MA. Increased risk of pancreatic cancer in melanoma-prone kindreds with p16INK4 mutations. N Engl J Med 1995;333:970–4 [DOI] [PubMed] [Google Scholar]

[R11] 11.Goldstein AM, Chan M, Harland M, Hayward NK, Demenais F, Bishop DT, Azizi E, Bergman W, Bianchi-Scarra G, Bruno W, Calista D, Albright LA, Chaudru V, Chompret A, Cuellar F, Elder DE, Ghiorzo P, Gillanders EM, Gruis NA, Hansson J, Hogg D, Holland EA, Kanetsky PA, Kefford RF, Landi MT, Lang J, Leachman SA, MacKie RM, Magnusson V, Mann GJ, Bishop JN, Palmer JM, Puig S, Puig-Butille JA, Stark M, Tsao H, Tucker MA, Whitaker L, Yakobson E. Features associated with germline CDKN2A mutations: a GenoMEL study of melanoma-prone families from three continents. J Med Genet 2007;44:99–106 [DOI] [PMC free article] [PubMed] [Google Scholar]

[R12] 12.Soufir N, Avril MF, Chompret A, Demenais F, Bombled J, Spatz A, Stoppa-Lyonnet D, Benard J, Bressac-de Paillerets B. Prevalence of p16 and CDK4 germline mutations in 48 melanoma-prone families in France. The French Familial Melanoma Study Group. Hum Mol Genet 1998;7:209–16 [DOI] [PubMed] [Google Scholar]

[R13] 13.Pjanova D, Engele L, Randerson-Moor JA, Harland M, Bishop DT, Bishop JA Newton, Taylor C, Debniak T, Lubinski J, Kleina R, Heisele O. CDKN2A and CDK4 variants in Latvian melanoma patients: analysis of a clinic-based population. Melanoma Res 2007;17:185–91 [DOI] [PubMed] [Google Scholar]

[R14] 14.Soufir N, Ollivaud L, Bertrand G, Lacapere JJ, Descamps V, Vitoux D, Lebbe C, Wolkenstein P, Dupin N, Saiag P, Basset-Seguin N, Grandchamp B. A French CDK4-positive melanoma family with a co-inherited EDNRB mutation. J Dermatol Sci 2007;46:61–4 [DOI] [PubMed] [Google Scholar]

[R15] 15.Majore S, De Simone P, Crisi A, Eibenschutz L, Binni F, Antigoni I, De Bernardo C, Catricala C, Grammatico P. CDKN2A/CDK4 molecular study on 155 Italian subjects with familial and/or primary multiple melanoma. Pigment Cell Melanoma Res 2008;21:209–11 [DOI] [PubMed] [Google Scholar]

[R16] 16.Pjanova D, Molven A, Akslen LA, Engele L, Streinerte B, Azarjana K, Heisele O. Identification of a CDK4 R24H mutation-positive melanoma family by analysis of early-onset melanoma patients in Latvia. Melanoma Res 2009;19:119–22 [DOI] [PubMed] [Google Scholar]

[R17] 17.Nikolaou V, Kang X, Stratigos A, Gogas H, Latorre MC, Gabree M, Plaka M, Njauw CN, Kypreou K, Mirmigi I, Stefanaki I, Tsao H. Comprehensive mutational analysis of CDKN2A and CDK4 in Greek patients with cutaneous melanoma. Br J Dermatol 2011;165:1219–22 [DOI] [PMC free article] [PubMed] [Google Scholar]

[R18] 18.Ghiorzo P, Bonelli L, Pastorino L, Bruno W, Barile M, Andreotti V, Nasti S, Battistuzzi L, Grosso M, Bianchi-Scarra G, Queirolo P. MC1R variation and melanoma risk in relation to host/clinical and environmental factors in CDKN2A positive and negative melanoma patients. Exp Dermatol 2012;21:718–20 [DOI] [PubMed] [Google Scholar]

[R19] 19.Coleman KG, Wautlet BS, Morrissey D, Mulheron J, Sedman SA, Brinkley P, Price S, Webster KR. Identification of CDK4 sequences involved in cyclin D1 and p16 binding. J Biol Chem 1997;272:18869–74 [DOI] [PubMed] [Google Scholar]

[R20] 20.Bartkova J, Lukas J, Guldberg P, Alsner J, Kirkin AF, Zeuthen J, Bartek J. The p16-cyclin D/Cdk4-pRb pathway as a functional unit frequently altered in melanoma pathogenesis. Cancer Res 1996;56:5475–83 [PubMed] [Google Scholar]

[R21] 21.Rees JL. The melanocortin 1 receptor (MC1R): more than just red hair. Pigment Cell Res 2000;13:135–40 [DOI] [PubMed] [Google Scholar]

[R22] 22.Mitra D, Luo X, Morgan A, Wang J, Hoang MP, Lo J, Guerrero CR, Lennerz JK, Mihm MC, Wargo JA, Robinson KC, Devi SP, Vanover JC, D'Orazio JA, McMahon M, Bosenberg MW, Haigis KM, Haber DA, Wang Y, Fisher DE. An ultraviolet-radiation-independent pathway to melanoma carcinogenesis in the red hair/fair skin background. Nature 2012;491:449–53 [DOI] [PMC free article] [PubMed] [Google Scholar]

[R23] 23.Garcia-Borron JC, Sanchez-Laorden BL, Jimenez-Cervantes C. Melanocortin-1 receptor structure and functional regulation. Pigment Cell Res 2005;18:393–410 [DOI] [PubMed] [Google Scholar]

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PERMALINK

Melanoma prone families with CDK4 germline mutation: phenotypic profile and associations with MC1R variants

Hanne Eknes Puntervoll

Xiaohong R Yang

Hildegunn Høberg Vetti

Ingeborg M Bachmann

Marie Françoise Avril

Meriem Benfodda

Caterina Catricalà

Stéphane Dalle

Anne B Duval-Modeste

Paola Ghiorzo

Paola Grammatico

Mark Harland

Nicholas K Hayward

Hui-Han Hu

Thomas Jouary

Tanguy Martin-Denavit

Aija Ozola

Jane M Palmer

Lorenza Pastorino

Dace Pjanova

Nadem Soufir

Solrun J Steine

Alexander J Stratigos

Luc Thomas

Julie Tinat

Hensin Tsao

Rūta Veinalde

Margaret A Tucker

Brigitte Bressac-de Paillerets

Julia A Newton-Bishop

Alisa M Goldstein

Lars A Akslen

Anders Molven

Series information

Abstract

Background

Methods

Results

Conclusion

Introduction

Methods

Recruitment of CDK4 mutated melanoma families and data collection

Table 1.

DNA analysis of CDK4 and MC1R

Statistical analysis

Results

Phenotypic characteristics of melanoma patients in CDK4 families

Table 2.

Table 3.

MC1R variants

Table 4.

Discussion

Supplementary Material

Acknowledgments

Footnotes

References

Associated Data

Supplementary Materials

ACTIONS

PERMALINK

RESOURCES

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