GEO Accession viewer

NCBI > GEO > Accession Display

Not logged in | Login

GEO help: Mouse over screen elements for information.

Series GSE3292

Query DataSets for GSE3292

Status

Public on Nov 28, 2005

Title

Gene expression signature of HPV in head and neck squamous cell carcinoma

Organism

Homo sapiens

Experiment type

Expression profiling by array

Summary

Introduction: Human Papilloma Virus (HPV) is associated with a subset of head and neck squamous cell carcinoma (HNSCC), between 15% and 35% of HNSCC harboring HPV, almost exclusively of subtype 16. Demographic and exposure differences between HPV-positive (+) and negative (-) HNSCCs suggest that HPV(+) tumors may constitute a subclass with different biology, while clinical differences have also been observed. In this study, gene expression profiles of HPV(+) and (-) tumors were compared to further explore the biological effect of HPV in HNSCC. Methods: Thirty-six HNSCC tumors were analyzed for gene expression using Affymetrix Human 133U Plus 2.0 GeneChip and for HPV using consensus primers for HPV L1, E6 and E7 by PCR and RT-PCR. Results: Eight (22%) of 36 tumors were positive for HPV, all of the HPV 16 subtype, and the HPV positive samples also expressed viral HPV E6 mRNA determined by RT-PCR. Patients with HPV(+) HNSCCs were on average younger than those with HPV(-) tumors (mean age 50.2 vs. 58.7). Statistical analysis using Significance Analysis of Microarrays (SAM) based on HPV status as a supervising parameter resulted in a list of 91 genes that were differentially expressed with statistical significance. Results for a sub-set of these genes were verified by RT-PCR. Genes highly expressed in HPV(+) samples included cell cycle regulators (p16INK4A, p18 and CDK2) and transcription factors (TAF7L, RFC4, RPA2 and TFDP2). The microarray data were also investigated using DIGMap to map genes by chromosomal location. A large number of genes on chromosome 3q24-qter was found to be overrepresented in HPV(+) tumors. Conclusion: The gene expression profile associated with HPV reflects alterations in cell cycle and proliferation signals. Further investigation of differentially expressed genes may reveal the unique pathways in HPV(+) tumors that may explain the different natural history and biological properties of these tumors. These properties may be exploited as a target of novel therapeutic agents in HNSCC treatment.
Keywords: HPV, HNSCC, head and neck cancer, human, human papilloma virus

Overall design

Patient selection and specimen collection. Thirty-six freshly frozen tumor samples were prospectively collected from patients undergoing surgery or biopsy for HNSCC at the University of North Carolina (UNC) at Chapel Hill (21 patients) and Vanderbilt University (15 patients). All tissues were snap-frozen in liquid nitrogen within 30 minutes of surgical resection or biopsy, and kept at -80oC until further processing. All patients consented to participation in this study under protocols approved by IRB at the two institutions.
HPV detection and DNA sequencing. Tumor DNAs were tested for the presence of HPV DNA using a previously established PCR-based method [11]. This method employs degenerate PCR primers (MY09 and MY11, WD72/76 and WD66/67/154) that are designed to represent highly conserved HPV L1 and E6 sequences present in all major types of HPV. In addition, all HPV-positive samples were also tested with a HPV16-specific PCR for E7 (primer A: 5’-GGA CCG GTC GAT GTA TGT CT-3’ and primer B: 3’-TAA AAC CAT CCA TTA CAT CCC G-5’). Optimal conditions for this combined PCR were determined using DNA from the cervical carcinoma cell line SiHa, which harbors on average 2 copies of HPV16 DNA per cell [11]. Other positive control cell lines were CaSki (HPV16) and HeLa (HPV18). For each case, 200 nanograms of tumor DNA were tested for the presence of HPV DNA. PCR samples which showed amplification products indicating the presence of HPV were purified using PCR purification columns (Qiagen, Valencia, CA) and subjected to bi-directional sequence analysis. In all of such cases, a positive identification of the HPV type could be made.
RNA isolation and DNA microarray analysis. Each tumor was examined by H&E staining to ensure presence of tumor and enriched by macrodissection to achieve a minimum of 70% tumor cells in each preparation. Total RNA was purified from frozen tumors using Qiagen RNeasy Mini Kit according to the manufacturer’s recommendations (Qiagen, Valencia, CA) using approximately 10-20 milligram of wet tissue from each sample. Fifty nanograms of the total RNA was amplified using NuGen RNA Amplification kit (NuGen, San Carlos, CA) and labeled ENZO BioArray High Yield RNA Transcript Labeling Kit (Affymetrix, Santa Clara, CA) according to the manufacturer's recommendations. Fifteen micrograms of biotin-labeled aRNA was fragmented and the quality of the RNA was reconfirmed using the Agilent RNA 6000 Nano LabChip Kit and Agilent 2100 bioanalyzer. The fragmented, biotin-labeled aRNA was combined with the hybridization mix and loaded on to the Affymetrix Human Genome U133 plus 2.0 GeneChip. After hybridization, the GeneChip was washed, stained with Strepavidin/phycoerythrin conjugate and biotinylated antibody, and scanned according to the manufacturer's recommendations. The raw microarray data was normalized using Perfect Match software for further statistical analyses.

Contributor(s)

Slebos R, Yi Y, Ely K, Carter J, Evjen A, Zhang X, Shyr Y, Murphy BM, Cmelak AJ, Burkey BB, Netterville JL, Levy S, Yarbrough WG, Chung CH

Citation(s)

16467079, 16943533

Submission date

Sep 12, 2005

Last update date

Mar 25, 2019

Contact name

Christine H. Chung

E-mail(s)

christine.chung@vanderbilt.edu

Phone

615-322-4967

Fax

615343-7602

Organization name

Vanderbilt University

Department

Internal Medicine

Lab

Chung

Street address

777 PRB

City

Nashville

State/province

ZIP/Postal code

37232-6307

Country

USA

Platforms (1)

GPL570

[HG-U133_Plus_2] Affymetrix Human Genome U133 Plus 2.0 Array

Samples (36)

More...

GSM73653	VU HNSCCV300142
GSM73654	VU HNSCCV300171
GSM73655	VU HNSCCV300251

Relations

BioProject

PRJNA92797

Significant Genes List header descriptions
Rank
Gene Name
Gene ID
Fold Change

Data table
Rank	Gene Name	Gene ID	Fold Change
Increased in HPV positive
1	233320_at	Homo sapiens LOC374817 (LOC374817), mRNA ---	5.5257
2	1557570_a_at	Homo sapiens, clone IMAGE:5244459, mRNA ---	3.2382
3	220325_at	TAF7-like RNA polymerase II, TATA box binding protein (TBP)-associated factor, 50kDa TAF7L	3.3099
4	205691_at	synaptogyrin 3 SYNGR3	2.5369
5	211156_at	cyclin-dependent kinase inhibitor 2A (melanoma, p16, inhibits CDK4) CDKN2A	5.2947
6	226832_at	Homo sapiens, clone IMAGE:5286726, mRNA ---	3.6660
7	231164_at	Homo sapiens, clone IMAGE:5271371, mRNA ---	3.7015
8	201756_at	replication protein A2, 32kDa RPA2	2.8151
9	241730_at	myoneurin MYNN	2.3719
10	1558217_at	hypothetical protein FLJ31952 FLJ31952	2.8412
11	206526_at	DKFZP566F0546 protein DKFZP566F0546	2.6313
12	230011_at	hypothetical protein MGC40042 MGC40042	2.2832
13	230301_at	hypothetical protein LOC340277 LOC340277	2.4832
14	238977_at	MCM6 minichromosome maintenance deficient 6 (MIS5 homolog, S. pombe) (S. cerevisiae) MCM6	2.7490
15	236236_at	Homo sapiens cDNA FLJ42662 fis, clone BRAMY2019546 ---	3.1076
16	204023_at	replication factor C (activator 1) 4, 37kDa RFC4	3.6455
17	225768_at	nuclear receptor subfamily 1, group D, member 2 NR1D2	2.5845
18	226456_at	hypothetical protein MGC24665 MGC24665	3.6016
19	205222_at	enoyl-Coenzyme A, hydratase/3-hydroxyacyl Coenzyme A dehydrogenase EHHADH	2.9072

Total number of rows: 94

Table truncated, full table size 6 Kbytes.

Patient Data header descriptions
Institute	VU: Vanderbilt University; UNC: University of North Carolina at Chapel Hill
ID
Age
Sex	M: Male; F: Female
Race	W: White; B: Black; O: Other
Site	HP: Hypopharynx; L: Larynx; OC: Oral Cavity; OP: Oropharynx
Tobacco	0 = no; 1 = yes
Alcohol	0 = no; 1 = yes; . = missing data
cStage	Clinical Stage
cStage	Clinical Stage
cLN	Clinical Cervical Lymph Nodes
pStage
pTNM
Grade
HPV

Data table
Institute	ID	Age	Sex	Race	Site	Tobacco	Alcohol	cStage	cStage	cLN	pStage	pTNM	Grade	HPV
VU	300142	68	F	W	OC	1	0	3	T3N0M0	0	1	T1N0M0	Moderate	Negative
VU	300148	50	M	W	L	0	0	3	T3N0M0	0	3	T3N0M0	Moderate	Positive
VU	300171	42	M	W	OP	0	0	4	T4N2cM0	1	4	T4N2cM0	Moderate	Positive
VU	300251	77	M	O	OP	1	1	4	T3N3M0	1	4	T3N3M0	Moderate	Negative
VU	300373	77	F	W	OC	0	0	1	T1N0M0	0	1	T1N0M0	Well	Negative
VU	300383	71	F	W	OC	1	0	4	T4N1M0	1	.	.	Moderate	Negative
VU	300400	89	M	B	L	0	0	3	T3N0M0	0	3	T3N0M0	Moderate	Negative
VU	300423	41	M	W	L	1	0	3	T3N0M0	0	3	T3N0M0	Moderate	Negative
VU	300431	65	M	W	OP	1	0	3	T3N1M0	1	3	T3N1M0	Poor	Positive
VU	300520	47	M	W	OP	1	1	3	T3N1M0	1	3	T3N1M0	Well	Positive
VU	300533	73	F	B	OC	1	0	4	T2N2bM0	1	4	T4N2bM0	Moderate	Negative
VU	300637	69	M	W	OC	1	1	3	T2N1M0	1	3	T1N1M0	Moderate	Negative
VU	300663	47	F	W	OC	1	0	2	T2N0M0	0	2	T2N0M0	Moderate	Negative
VU	300688	47	M	W	OC	1	1	4	T2N2bM0	1	4	T2N2bM0	Moderate	Negative
VU	300710	58	M	W	OC	1	1	1	T1N0M0	0	3	T1N1M0	Moderate	Negative
UNC	318	56	M	B	L	1	1	4	T4N0M0	0	4	T4N1M0	Moderate	Negative
UNC	10291	72	M	B	L	1	1	4	T3N2aM0	1	4	T3N2aM0	Poor	Negative
UNC	10393	47	M	O	OP	1	0	4	T3N2bM0	1	4	T3N2bM0	Moderate	Negative
UNC	10394	48	M	W	OP	1	1	4	T1N3M0	1	4	T2N3M0	Moderate	Positive
UNC	10446	59	M	B	L	1	1	3	T3N0M0	0	4	T3N2cM0	Poor	Negative

Total number of rows: 36

Table truncated, full table size 2 Kbytes.

Download family	Format
SOFT formatted family file(s)	SOFT
MINiML formatted family file(s)	MINiML
Series Matrix File(s)	TXT

Supplementary file	Size	Download	File type/resource
GSE3292_RAW.tar	169.9 Mb	(http)(custom)	TAR (of CEL)