Steatocystoma multiplex is associated with the R94C mutation in the KRTl7 gene.

Steatocystoma multiplex (SM) is an uncommon disorder, characterized by numerous skin‑colored subcutaneous cysts. A number of SM pedigrees have been identified with mutations in the keratin 17 (KRT17) gene. The present study examined a four‑generation Chinese pedigree with an autosomal dominant mode of inheritance and examined its genetic basis. A review of the literature on KRT17 gene mutations in the SM pedigree was also performed to investigate the KRT17 gene mutation and genotype‑phenotype correlation. Exon 1 of the KRTl7 gene was amplified using polymerase chain reaction (PCR) from genomic DNA obtained, which was obtained from 25 family members in the selected Chinese pedigree and from 100 unrelated control individuals. The DNA was then subjected to automatic DNA sequencing. Genealogical investigations demonstrated an autosomal dominant pattern, and direct sequencing of the PCR product revealed a heterozygous mutation, c.280C/T (R94C), which was located in exon 1 of the KRT17 gene in all 10 affected family members. The mutation was not identified in the 15 unaffected family members or in the 100 unrelated control individuals. Therefore, the present study identified a causative mutation in the KRT17 gene in a large Chinese SM pedigree, exhibiting autosomal dominance. A review of the literature suggested that, in addition to the mutation factor, other modifying factors contribute to the phenotype of familial SM.

Introduction

Steatocystoma multiplex (SM; OMIM184500) is an uncommon disorder, which is characterized by numerous skin-colored subcutaneous cysts that originate from the pilosebaceous duct. Although a number of sporadic cases have been reported, SM is considered to be an autosomal dominant disorder. Certain SM pedigrees have been identified with mutations in the keratin 17 (KRT17) gene, which have also been reported in patients with pachyonychia congenital type 2 (1). These mutations are highly conserved at the beginning sequence of helix 1A in the KRT17 gene, at which any substitution or deletion may lead to a distortion of the α-helical structure at the beginning of the 1A domain (2). Mutations in this location are considered to have a significant effect on the assembly and/or integrity of the keratin cytoskeleton in cells (3). The tissues affected include the outer root sheath of the hair follicle, sebaceous glands, nail beds and other appendages (4), which explain the phenotypes of nail dystrophy and steatocystoma multiplex that are observed in patients with pachyonychia congenital type 2 (3,5).

The present study investigated a Chinese four-generation autosomal dominant SM pedigree in order to identify the causative mutation by means of polymerase chain reaction (PCR) analysis and DNA sequencing. In addition, a literature review of KRT17 gene mutations in SM pedigrees was performed to investigate the KRTl7 gene mutation and the genotype-phenotype correlation.

Patients and methods

Pedigree analysis

A four-generation Chinese SM pedigree with an autosomal dominant mode of inheritance was examined. The genealogical tree of this SM pedigree is shown in Fig. 1. The proband (III-13) was a 26-year-old male of Chinese Han-nationality, with the symptom of a gradual appearance of multiple skin-colored nodules on his whole body for >20 years. The lesions gradually developed in size and number at infancy, and became severe and obvious during puberty. The lesions were asymptomatic, however, were of cosmetic concern. When punctured, the cysts discharged yellowish, oily material and healed with a scar. The proband was in good general health and his routine laboratory investigations were within normal limits. On physical examination, multiple, skin-colored, firm, globoid nodules, measuring between 2 and 30 mm in diameter on the face, neck, chest, abdomen, arms and legs of the proband were identified (Fig. 2). The nail, palmoplantar areas, mouth, tongue and teeth were all normal. Histological examination of these lesions revealed that the cyst wall was composed of several layers of epithelial cells, accompanied by sebaceous gland lobules (Fig. 3). On the basis of these findings, the diagnosis of SM was made. Another nine affected members of his family reported a similar history, namely, his grandfather (I-1), father (II-3), uncle (II-9), three sisters (III-12,16,17), two nieces and one nephew (IV-23,24,25). None of these affected individuals exhibited any nail changes or any other skin, hair or mucosal abnormalities. The conditions of the patients varied and the condition of the female patients were comparatively milder in this family. The remaining members of this family had no history of SM.

Figure 1

Four generation pedigree (I–IV) of the family comprising a number of individuals affected with SM. The squares indicate male family members and the circles indicate female family members. Black symbols indicate individuals exhibiting symptoms of SM, whereas white symbols indicate healthy, unaffected individuals. The proband (III-13) in the present study is indicated by an arrow. * indicates individuals from whom DNA was not obtained. SM, steatocystoma multiplex.

Figure 2

Steatocystoma multiplex lesions located on the neck and chest of the proband.

Figure 3

Hematoxylin and eosin stained histological section of a steatoma from the proband individual diagnosed with steatocystoma multiplex. A steatocystoma with sebaceous gland lobules in the cyst wall are present (magnification, ×40).

Mutation analysis

Ethical approval was obtained from the ethics committee of Hainan Provincial Hospital of Skin Disease (Haikou, China) and written informed consent was also obtained. The genomic DNA was extracted from peripheral blood samples of 25 individuals within the family (10 affected and 15 unaffected family members) using a QIAamp blood-tissue kit (Qiagen, Hilden, Germany), according to the manufacturer's instructions. The exon 1 coding sequence of KRT17 (GenBank Entry: NM_000422) was amplified by polymerase chain reaction (PCR) using primer pairs designed with Primer3 (http://frodo.wi.mit.edu/primer3). The primer sequences were as follows: Forward 5′-ATGGAAACAGAGGAGCA-3′ and reverse 5′-CCTGACTCAGCTTGCTGT-3′. The DNA template (100 ng) was mixed in a solution containing 1X PCR buffer, consisting of 100 mM Tris-HCl (pH 8.3) and 500 mM KCl, 1.5 mM MgCl2, 50 µM dNTPs, 10 pmol of each primer, and 2.5 units of Taq DNA polymerase (Promega Corporation, Madison, WI, USA), in a final reaction volume of 30 µl. Amplification was performed in an initial denaturation at 95ºC for 1 min, followed by 35 cycles of denaturing at 95ºC for 40 sec, annealing at 58ºC for 40 sec and extension at 72ºC for 1 min, with a final extension at 72ºC for 3 min. This resulted in a 830 bp fragment with the use of Eppendorf Mastercycler Gradient PCR (Eppendorf, Hamburg, Germany). The PCR samples contained 5% dimethyl sulfoxide to amplify the two fragments. The PCR products were purified using a Promega Wizard® SV 96 PCR Clean-up kit (Promega Corporation), according to the manufacturer's instructions, eluted in 100 µl H2O and directly sequenced using an ABI Prism 377 DNA sequencer (Applied Biosystems Life Technologies, Foster City, CA, USA). The mutation was confirmed by performing identical PCR and sequencing in 100 unrelated control individuals. Geneious version R8 software (Biomatters, Ltd., Auckland, New Zealand) was used to compare sequences.

Literature review

A literature review of KRT17 gene mutations in SM pedigrees was performed through searches of PubMed (http://www.ncbi.nlm.nih.gov/pubmed/), Ovid Medline (http://ovidsp.tx.ovid.com/sp-3.16.0a/ovidweb.cgi), EMBASE databases (http://www.embase.com) and China National Knowledge Infrastructure (http://www.cnki.net/). To the best of our knowledge, only seven types of KRT17 gene mutation in nine SM pedigrees have been reported in the literature (2,3,5–17) (Table I).

Table I

Synopsis of KRT17 mutations in SM pedigrees in Chinese non-Chinese populations from a review of previous studies.

Domain	Mutation	Phenotype	Heredity	Population	Reference
V1	S24L 71C>T	SM	Familial	Chinese	(6)
1A	N92H 274A>C	SM	Familial		(7)
1A	N92S 275A>G	SM	Familial	Chinese	(8)
		PC-2	Familial		(2)
			Familial		(3)
			Familial		(5)
			Familial & sporadic		(7)
			Familial		(9)
			Familial		(10)
			Familial		(11)
			Familial		(12)
1A	R94H 281	SM	Familial		(7)
	G>A	SM	Familial	Chinese	(8)
		PC-2	Sporadic		(13)
1A	R94C 280	SM	Familial	Chinese	(14)
	C>T	SM	Familial		(15)
		PC-2	Familial		(3)
			Familial		(12)
1A	R94G 280C>G	SM	Familial	Chinese	(16)
2B	L371P 1112T>C	SM	Familial		(17)

SM, steatocystoma multiplex; PC-2, pachyonychia congenital type 2.

Results

Identification of the large SM pedigree with autosomal dominant inheritance

Starting from the aforementioned proband, a four-generation pedigree was constructed through extensive genealogical investigation (Fig. 1). A total of 10 (five male and five female) of the 27 family members exhibited similar clinical manifestations. The availability of the phenotypic data led to the establishment of a mode of autosomal dominant inheritance in this large pedigree.

Identification of the causative gene using PCR and DNA sequencing

By direct sequencing of the KRT17 genomic PCR products, a heterozygous mutation (c.280C>T) was identified in exon 1 of the KRT17 gene in all 10 affected family members, which causes an arginine to cysteine amino acid substitution at codon 94 (R94C). No such mutation was identified in any of the 15 unaffected family members or in the 100 unrelated control individuals (Fig. 4).

Figure 4

DNA sequence electrophoretogram of the DNA obtained from the proband (III-13) and the proband's mother (II-4). (A) DNA sequence electrophoretogram of the heterozygous mutation R94C (c.280C>T; GenBank entry: NM_000422) of KRT17 in the proband (indicated by the arrow). (B) No equivalent mutation was detected in the proband's mother.

Discussion

The present study successfully identified the heterozygous mutation, c.280C>T (R94C) in exon 1 of the KRT17 gene as the cause of SM in the large, four-generation Chinese pedigree examined, and was revealed to be an autosomal dominant form.

By reviewing the previous literature (2,3,5–17), it was revealed that seven mutations have been previously reported in nine families with SM (Table I). These independent findings provided support for the involvement of the KRT17 gene in SM. A total of three of seven previously reported mutations, N92S, R94H and R94C, were associated with SM and PC-2, while the other four, S24L, N92H, L371P and R94G, were only associated with SM. S24L, N92S, R94H, R94C and R94G were reported in seven Chinese families with SM, and the R94C mutation has been detected previously in two families with SM and two families with PC-2 (3,12,14,15), which was the second time that SM was observed in a Chinese family. The majority of mutations in familial SM have been reported within the highly conserved helix boundary domains at the end of the α-helical rod domain of keratin (7,8,14–16).

According to the data obtained in previous studies, presented in Table I, a number of different mutations may lead to the identical clinical phenotype in SM, while the same mutations may cause different phenotypic variations in patients with SM or PC-2. Previous studies indicated variable onset ages of subcutaneous cysts in different SM pedigrees or SM family members. For example, with the R94C mutation, the onset of sebaceous cysts occurred in the same year as birth in certain individuals, however, no sebaceous cysts occurred until the second decade in other individuals (14,15). This finding suggests that the genotype-phenotype correlation of SM may be determined, not only by the site and type of the KRT17 gene mutation, but also by other modifying factors. According to previous studies, androgenic stimulation and environmental factors have been suggested as the possible reasons (2,3,18). In the pedigree examined in the present study, the early onset of clinical manifestations, aggravation during puberty, variable severity of different patients and milder symptoms in female family members appeared to support the above-mentioned hypothesis that there are other modifying factors contributing to the phenotype of familial SM.

In conclusion, using PCR and DNA sequencing, the present study identified a causative mutation, c.280C>T (R94C), in the KRT17 gene in a large Chinese SM pedigree with an autosomal dominant form. A review of the findings of previous studies suggested that, with the exception of the mutation factor, other modifying factors contribute to the phenotype of familial SM. This observation may assist in elucidating the molecular consequences of the KRT17 mutation in familial SM and may offer further insight into the correlation between KRT17 gene mutations and genotype-phenotype correlation.