Introduction

Oncology Letters

1792-1074 1792-1082

D.A. Spandidos

10.3892/ol.2016.5264

OL-0-0-5264

Articles

Folate deficiency and aberrant expression of cell adhesion molecule 1 are potential indicators of prognosis in laryngeal squamous cell carcinoma

Chang

Hao

1 Ma

Min

1 Ma

Rui

2 Zhang

Chao

1 Zeng

Wei

1 Xing

Lu Qi

1Department of Otolaryngology, The First Affiliated Hospital, College of Clinical Medicine of Henan University of Science and Technology, Luoyang, Henan 471003, P.R. China 2Department of Central Laboratory, Eye & ENT Hospital of Fudan University, Shanghai 200032, P.R. China 3Department of Pathology, The First Affiliated Hospital and College of Clinical Medicine of Henan University of Science and Technology, Luoyang, Henan 471003, P.R. China

Correspondence to: Dr Min Ma, Department of Otolaryngology, The First Affiliated Hospital, and College of Clinical Medicine of Henan University of Science and Technology, 24 Jing Hua Road, Luoyang, Henan 471003, P.R. China, E-mail: minma33@sina.com

12 2016

14 10 2016

12 6 4510 4514 10072015 19082016

2016

This is an open access article distributed under the terms of the Creative Commons Attribution-NonCommercial-NoDerivs License, which permits use and distribution in any medium, provided the original work is properly cited, the use is non-commercial and no modifications or adaptations are made.

The etiology of laryngeal squamous cell carcinoma (LSCC) has not yet been adequately examined. Therefore, the present study aimed to investigate the association between serum folate deficiency and abnormal expression of the cell adhesion molecule 1 (CADM1) protein in the progression of LSCC. Samples were collected from 60 patients with LSCC and 30 healthy people. Radioimmunoassays and immunohistochemical staining were performed to measure serum folate levels and CADM1 protein expression, respectively. The results demonstrated that CADM1 expression in LSCC specimens was significantly lower than in adjacent normal tissues (χ²=28.229, P<0.001), which was associated with histological differentiation and clinical stage (P=0.010 and 0.020, respectively). Levels of serum folate in patients with LSCC were significantly lower than those observed in healthy individuals (P=0.002). Furthermore, TSLCl expression and serum folate levels were positively correlated in LSCC (r=0.642, P=0.001). Thus, the present study determined that decreased CADM1 protein expression and low levels of serum folate were correlated with an increased severity of LSCC.

folate cell adhesion molecule 1 laryngeal squamous cell carcinoma

Introduction

Laryngeal squamous cell carcinoma (LSCC) is one of the most common malignant tumors identified in the head and neck. LSCCs account for 90% of all larynx carcinomas, ~90% of which are in males. Furthermore, the majority of patients are aged between 40 and 60-years-old (1). At present, there is no specific biomarker for LSCC diagnosis and prognosis. Thus, the current study aimed to examine potential biomarkers that could improve the early diagnosis of LSCC.

The cell adhesion molecule 1 (CADM1) gene encodes a membrane protein, which is silenced in ~44% of patients with non-small cell lung cancer and 30–60% of those with other types of cancer (2). Previous studies have identified two mechanisms of CADM1 inactivation: Promoter hypermethylation and loss of heterozygosity (3–5). Furthermore, it has been demonstrated that the CADM1 protein participates in a number of biological functions, including synapse formation, cell adhesion and tumor suppression (6). In several types of tumors, the absence of CADM1 expression is closely related to invasive tumor behavior (6–9). However, the role of CADM1 in LSCC remains largely unknown. To investigate the association between CADM1 protein expression and the development of LSCC, 60 surgically resected specimens were collected and assessed for loss of the CADM1 protein using immunohistochemistry. Subsequently, the association of CADM1 protein expression with LSCC clinicopathological parameters and the histological growth pattern of the tumors were investigated.

Folate is a water-soluble B vitamin that mediates one-carbon metabolism in vivo and serves multiple functions in physiological processes. Folate provides one-carbon groups for DNA replication, epigenetic modifications and DNA mutation prevention, thus protecting against tumorigenesis (10). Additionally, tetrahydrofolate synthesis in vivo requires folate for blood cell development and maturation (11). Folate deficiency is closely associated with glossitis, anemia and, in pregnancy, fetal neural tube defects (12). Previous studies have suggested that folate may aid cancer prevention (13,14), and several studies have demonstrated that a reduction in serum folate levels may be closely related to several types of cancer, including colorectal cancer (15–17). However, no similar report in LSCC was found in the literature. Therefore, it is necessary to investigate the relationship between serum folate levels and cancer progression and prognosis. The present study aimed to investigate the underlying association between folate deficiency and CADM1 protein expression in LSCC.

Patients and methods <sec> <title>Patients and tissue specimens

A total of 60 pairs of LSCC and precancerous specimens were collected from patients treated at the Department of Otolaryngology, Head and Neck Surgery at the First Affiliated Hospital of Henan University of Science and Technology (Luoyang, China) between September 2011 and September 2014. The control group consisted of 30 healthy volunteers whose blood was collected during routine health examinations. The ratio of patients to healthy volunteers was 1:2. Precancerous tissues were defined as the laryngeal mucosa 2 cm from the edge of the cancerous site. Patients had undergone preoperative partial or total laryngectomy without radical and chemical therapies. Patients with megaloblastic anemia or other types of anemia, upper gastrointestinal tract diseases, and those treated with any other surgical procedures, were excluded. Patients with a history of smoking, oral contraceptive use or those who had taken B vitamins in the past 6 months were also excluded from the current study. The Ethics Committee of the First Affiliated Hospital of Henan University of Science and Technology (Luoyang, China) approved the use of human tissues for the current study. All patients and volunteers provided written informed consent to participate.

Immunohistochemistry

Expression of the CADM1 protein was tested using an Immunohistochemical S-P kit against CADM1 (Kangwei Bio, Ltd., Beijing, China), according to the manufacturer's protocol. A rabbit polyclonal antibody against CADM1 (1:100 dilution, cat. no. Rs-1147R) was purchased from Kangwei Bio, Ltd. Tissues were fixed with 10% formaldehyde solution, cut into 3-µm sections, embedded in paraffin blocks and subsequently incubated with the polyclonal antibody at 4°C overnight (>14 h). Sections were subsequently incubated with biotinylated goat anti-rabbit immunoglobulin G (1:100 dilution, cat. no. CW2035S; Kangwei Bio, Ltd.) for 40 min at room temperature. Phosphate-buffered saline was used as a negative control. 3,3′-diaminobenzidine was used to stain the sections and hematoxylin was used as a counterstain to highlight the cytoblasts and background color. Each section was observed in 10 random fields under ×200 magnification (18). The score was calculated by adding the scores for intensity (weak=1, moderate=2, intense=3) and proportion (5%=1, 6–24%=2, 25–49%=3, 50–74%=4, ≥75%=5) of positively stained cells (19). Scores of ≥2 were considered positive. Two independent pathologists assessed each slide.

Radioimmunoassay

Whole blood samples (6 ml) were drawn from a peripheral vein of each participant after overnight fasting. Following the centrifugation of whole blood samples at 300 × g for 15 min, serum samples were collected and stored at −80°C until analysis. Serum folate levels were tested using radioimmunoassay quantification with a commercial kit for measurement of folate (Shanghai Ruiqi Bio-Technology, Co., Ltd., Shanghai, China), according to the manufacturer's instructions.

Statistical analysis

Data were analyzed using Student's t-test, χ² test, one-way analysis of variance (ANOVA), Student-Newman-Keuls test, Fisher's exact test and Spearman's rank correlation coefficient. SPSS version 16.0 for Windows (SPSS Inc., Chicago, IL, USA) was used to analyze all results. P<0.05 was considered to indicate a statistically significant difference.

Results <sec> <title>Expression of the CADM1 protein in LSCC

CADM1 protein expression was detected via immunohistochemical analysis of 60 malignant squamous cells of larynx tumors and 60 corresponding healthy adjacent non-neoplastic tissues, which were examined as a comparison. The results demonstrated that 47 specimens (78%) of adjacent normal tissues expressed CADM1 protein. By contrast, only 12 tumor specimens (20%) expressed the CADM1 protein (P<0.001; Table I). The associations among CADM1 expression patterns in the tumors, serum folate levels and patient clinical characteristics are presented in Table II. Positive staining indicated that CADM1 was primarily located in the cytoplasm in the adjacent normal tissues, but was absent in the tumor tissues (Fig. 1A and B, indicated by shapes). Expression of the CADM1 protein was not correlated with patient age or anatomic localization (P=1.000 and 0.386, respectively), but was correlated with histological differentiation and clinical stage (P=0.010 and 0.020, respectively; Table II).

Associations among patient characteristics, expression of CADM1 and serum folate levels

One-way ANOVA was used to determine differences in the serum folate levels among LSCC tissues with different clinical characteristics, including age, clinical stage, histological differentiation and anatomic localization. The differences were statistically significant among tumor tissues with different clinical stages, histological differentiation and anatomic localizations (P=0.001, 0.001 and 0.001, respectively; Table II). To further clarify the relationship between serum folate levels and stage of LSCC, a Student-Newman-Keuls test was used for multiple comparisons of clinical stage, histological differentiation and anatomic localization. The results indicated that serum folate levels decreased as tumor malignancy increased (Table III). Additionally, serum folate levels were significantly lower in patients with LSCC compared with healthy control subjects (P=0.002; Table IV). The spearman correlation analysis identified a significant correlation between CADM1 protein expression and serum folate levels (r=0.642, P=0.001). Therefore, folate deficiency may decrease the methylation of CADM1 promotor and regulate CADM1 expression. However, further studies are required to confirm this.

Discussion

In the present study, all included patients were male and most patients aged <50 years were TNM stage III or IV with higher serum folate levels, whereas patients aged >50 years were stages I–II with lower serum folate levels. The critical factor in the prognosis of LSCC is tumor metastasis, however, the etiopathogenesis of tumor metastasis remains largely unknown and may involve immune dysregulation. CADM1, located on chromosome 11q23.2, encodes a transmembrane protein from the immunoglobulin superfamily (20). Previous studies have demonstrated that CADM1 is a human tumor suppressor and mutations in its cytoplasmic domain have been linked to lung tumor cell metastasis, aggravated histological differentiation, clinical stage classification and a poor prognosis (6,21,22). The results of the present study were consistent with previous studies (23,24) and established that, as compared with adjacent non-neoplastic tissue, tumor tissues express lower levels of CADM1. This is important as CADM1 may serve a potential role in the diagnosis and prognosis of LSCC.

Duthie et al (25) affirmed the effect of folate deficiency on chromosome breaks and the risk of carcinogenesis. Furthermore, it has been determined that folate deficiency may decrease thymidine synthesis and stimulate uracil misincorporation into DNA (26,27). Homeostasis of folate is critical to DNA stability and integrity, as well as the repair of damaged DNA, and folate supplementation may have a protective effect against cancer (15,16,28,29). The results of the current study demonstrated that serum folate levels in patients with LSCC were markedly lower than those in healthy individuals and decreased with the deterioration in the degree of tumor malignancy. This indicates that low serum folate levels may be associated with the increased malignancy of LSCC.

The results of the present study suggested that there was a significant association between CADM1 protein expression and serum levels of serum folate in patients with LSCC (r=0.642, P=0.001). CADM1 expression varied among different anatomic localizations; therefore, this relationship may result from the different malignant degrees and carcinoma progression. However, the unique microenvironments of different anatomical localizations may also contribute to the difference. Therefore, further studies are required to understand why these differences occur.

The analysis demonstrated that the decline of serum folate levels may be the cause of low CADM1 expression in LSCC tumor tissue. It was observed that a significant proportion of LSCC patients had low serum folate levels. Furthermore, as the severity of LSCC increased, serum folic acid levels decreased. Therefore, folate deficiency may be associated with the excessive consumption of folic acid in the body (due to the increased energy needs of patients with cancer) during repair of the damaged CADM1 gene (17).

Folate is a critical factor of DNA methylation (29) and methylation of promoter DNA has been regarded as an important mechanism of CADM1 gene silencing (30). In the present study, CADM1 downregulation in LSCC tumor tissue was observed; however, the underlying mechanism was not investigated. Therefore, further clinical studies are necessary. In future studies, we intend to evaluate the effectiveness of serum folic acid supplementation in patients with LSCC and to identify the intrinsic relationship between folate and promoter methylation of the CADM1 gene.

Acknowledgements

This study was supported by the Provincial Science and Technology Foundation of Henan Province, China (grant no. 132102310029).

References 1

Huang

Wang

Kong

Practice of Otorhinolaryngology-Head and Neck Surgery2nd

People's Medical Publishing House

Bei Jing, China

2007

10.1016/j.otohns.2007.06.628

Murakami

Nobukuni

Tamura

Maruyama

Sekiya

Arai

Gomyou

Tanigami

Ohki

Cabin

Localization of tumor suppressor activity important in nonsmall cell lung carcinoma on chromosome 11q

Proc Natl Acad Sci USA95815381581998

10.1073/pnas.95.14.8153

9653156

Allinen

Peri

Kujala

Lahti-Domenici

Outila

Karppinen

Launonen

Winqvist

Analysis of 11q21-24 loss of heterozygosity candidate target genes in breast cancer: Indications of TSLC1 promoter hypermethylation

Genes Chromosomes Cancer343843892002

10.1002/gcc.10079

12112527

Fong

Kida

Zimmerman

Ikenaga

Smith

Loss of heterozygosity frequently affects chromosome 17q in non-small cell lung cancer

Cancer Res55426842721995

7671234

Zhou

Jiang

Ren

Yin

Feng

Liu

Tao

Yao

Frequent hypermethylation of RASSF1A and TSLC1 and high viral load of Epstein-Barr Virus DNA in nasopharyngeal carcinoma and matched tumor-adjacent tissues

Neoplasia78098152005

10.1593/neo.05217

16229803

Kuramochi

Fukuhara

Nobukuni

Kanbe

Maruyama

Ghosh

Pletcher

Isomura

Onizuka

Kitamura

TSLC1 is a tumor suppressor gene in human non-small cell lung cancer

Nat Genet274274302001

10.1038/86934

11279526

Murakami

Involvement of a cell adhesion molecule, TSLC1/IGSF4, in human oncogenesis

Cancer Sci965435522005

10.1111/j.1349-7006.2005.00089.x

16128739

Fukuhara

Kuramochi

Fukami

Kasahara

Furuhata

Nobukuni

Maruyama

Isogai

Sekiya

Shuin

Promoter methylation of TSLC1 and tumor suppression by its gene product in human prostate cancer

Jpn J Cancer Res Jun936056092002

10.1111/j.1349-7006.2002.tb01297.x

Jansen

Fukushima

Rosty

Walter

Altink

Heek

Hruban

Offerhaus

Goggins

Aberrant methylation of the 5′ CpG island of TSLC1 is common in pancreatic ductal adenocarcinoma and is first manifest in high-grade PanlNs

Cancer Biol Ther12932962002

10.4161/cbt.84

12432281

Kamen

Folate and antifolate pharmacology

Semin Oncol24(5 Suppl 18)S18-30S18-391997

Friso

Choi

Gene-nutrient interactions and DNA methylation

J Nutr132(8 Suppl)2382S2387S2002

12163697

Allen

Stabler

Savage

Lindenbaum

Metabolic abnormalities in cobalamin (vitamin B12) and folate deficiency

FASEB J7134413531993

7901104

Sie

Medline

van Weel

Sohn

Choi

Croxford

Kim

Effect of maternal and postweaning folic acid supplementation on colorectal cancer risk in the offspring

Gut60168716942011

10.1136/gut.2011.238782

21561879

Jennings

Willis

How folate metabolism affects colorectal cancer development and treatment; a story of heterogeneity and pleiotropy

Cancer Lett3562242302015

10.1016/j.canlet.2014.02.024

24614284

Kim

Role of folate in colon cancer development and progression

J Nutr13311Suppl 13731S3739S2003

14608107

Choi

Mason

Folate status: Effects on pathways of colorectal carcinogenesis

J Nutr132(8 Suppl)2413S2418S2002

12163703

Kim

Folate and carcinogenesis: Evidence, mechanisms, and implications

J Nutr Biochem1066881999

10.1016/S0955-2863(98)00074-6

15539274

Kuramochi

Fukuhara

Nobukuni

Kanbe

Maruyama

Ghosh

Pletcher

Isomura

Onizuka

Kitamura

TSLC1 is a tumor-suppressor gene in human non-small-cell lung cancer

Nat Genet274274302001

10.1038/86934

11279526

Yong

Yang

Suyila

Han

Yuan

Zhao

Expression and clinical implications of P53, P63, and P73 protein in malignant tumor of the parotid gland

Turk J Med Sci448758822014

10.3906/sag-1304-136

25539561

Yurdakul

Akyurek

Yilmaz

Karakaya

Memİş

Ozturk

Prognostic impact of matrix metalloproteinases (MMP-9 and MMP-2) and vascular endothelial growth factor expression in non-small cell lung cancer

Turk J Med Sci422812882012

Uchino

Ito

Wakayama

Koma

Okada

Ohbayashi

Iseki

Kitamura

Tsubota

Okita

Okada

Clinical implication and prognostic significance of the tumor suppressor TSLC1 gene detected in adenocarcinoma of the lung

Cancer98100210072003

10.1002/cncr.11599

12942568

Blount

Mack

Wehr

MacGregor

Hiatt

Wang

Wickramasinghe

Everson

Ames

Folate deficiency causes uracil misincorporation into human DNA and chromosome breakage: Implications for cancer and neuronal damage

Proc Natl Acad Sci USA94329032951997

10.1073/pnas.94.7.3290

9096386

Surace

Lusis

Murakami

Scheithauer

Perry

Gutmann

Loss of tumor suppressor in lung cancer-1 (TSLC1) expression in meningioma correlates with increased malignancy grade and reduced patient survival

J Neuropathol Exp Neurol63101510272004

10.1093/jnen/63.10.1015

15535129

Steenbergen

Kramer

Braakhuis

Stern

Verheijen

Meijer

Snijders

TSLC1 gene silencing in cervical cancer cell lines and cervical neoplasia

J Natl Cancer Inst962943052004

10.1093/jnci/djh031

14970278

Duthie

Grant

Narayanan

Increased uracil misincorporation in lymphocytes from folate-deficient rats

Br J Cancer83153215372000

10.1054/bjoc.2000.1481

11076664

Duthie

Narayanan

Brand

Pirie

Grant

Impact of folate deficiency on DNA stability

J Nutr132(8 Suppl)2444S2449S2002

12163709

Butterworth

Effect of folate on cervical cancer. Synergism among risk factors

Ann N Y Acad Sci6692932991992

10.1111/j.1749-6632.1992.tb17108.x

1332564

Mason

Levesque

Folate: Effects on carcinogenesis and the potential for cancer chemoprevention

Oncology (Williston Park)10172717361742–17441996

8953590

Murakami

Functional cloning of a tumor suppressor gene, TSLC1, in human non-small cell lung cancer

Oncogene21693669482002

10.1038/sj.onc.1205825

12362275

Fukami

Fukuhara

Kuramochi

Maruyama

Isogai

Sakamoto

Takamoto

Murakami

Promoter methylation of the TSLC1 gene in advanced lung tumors and various cancer cell lines

Int J Cancer10753592003

10.1002/ijc.11348

12925956

Figure 1.

Cell adhesion molecule 1 (CADM1) expression in laryngeal squamous cell carcinoma tumor tissue compared with adjacent normal tissue. (A) CADM1 expression in severe atypical hyperplasia tissue and the absence of its expression in the tumor (magnification, ×100). ▲=Severe atypical hyperplasia tissue, ●=tumor tissue. (B) CADM1 expression in mild atypical hyperplasia tissue and the absence of its expression in the tumor (magnification, ×100). ▲=Mild atypical hyperplasia tissue. ●=tumor tissue.

Table I.

Expression of the CADM1 protein in laryngeal squamous cell carcinoma and adjacent normal tissues.

		CADM1

Group	n	Positive	Negative	χ²	P-value
Tumors	60	12	48	28.229	0.001^a
Adjacent normal tissues	60	47	13

P<0.01; n, number of samples; CADM1, cell adhesion molecule 1.

Table II.

Associations among patient clinical characteristics, protein expression of CADM1 and serum folate levels.

Characteristic	n	P	N	Folic acid (ng/ml)	P-value: Fisher's exact test	P-value: One-way ANOVA
Age (years)
≥50	49	15	34	3.53±1.53
<50	11	3	8	2.36±0.98	1.000	0.058
TNM stage
I	27	12	15	3.69±1.45
II	17	6	11	3.65±1.57
III	11	0	11	2.44±1.32
IV	5	0	5	2.46±1.07	0.010^a	0.001^b
Histological differentiation
Well	34	15	19	3.85±1.33
Moderately	16	3	13	3.18±1.66
Poorly	10	0	10	1.95±0.86	0.010^a	0.001^b
Anatomic localization
Supraglottic	8	2	6	2.08±0.96
Glottic	39	14	25	3.86±1.45
Subglottic	13	2	11	2.94±1.23	0.386	0.001^b

P<0.05

P<0.01; n, number of patients; P, CADM1-positive cells; N, CADM1-negative cells; CADM1, cell adhesion molecule 1; ANOVA, analysis of variance; TNM, tumor-node-metastasis.

Table III.

Associations between serum folic acid levels in patients with laryngeal squamous cell carcinoma and clinical stage, histological differentiation and anatomic localization.

Clinical stage (TNM)	P-value	Histological differentiation and anatomic localization	P-value
I and II	0.610	1 and 2	0.110
I and III	0.002^a	1 and 3	0.001^b
I and IV	0.001^b	2 and 3	0.020^a
II and III	0.014^a	A and B	0.001^b
II and IV	0.004^b	A and C	0.160
III and IV	0.320	B and C	0.080

P<0.05

P<0.01; 1, well-differentiated; 2, moderately-differentiated; 3, poorly-differentiated; A, supraglottic; B, glottic; C, subglottic; TNM, tumor-node-metastasis.

Table IV.

Serum folic acid levels in patients with LSCC and healthy controls.

Group	n	Folic acid (ng/ml)
Healthy controls	30	4.40±1.47^a
Patients with LSCC	60	3.35±1.51

Data are presented as the mean ± standard deviation.

P=0.002. n, number of patients; LSCC, laryngeal squamous cell carcinoma.