Squamous Cell Carcinoma Clinical Trial
Official title:
Comparison of Detection of Human Papillomavirus on Tissue, Saliva and Serum
Human papillomavirus (HPV) is one of the most prevalent infections in the world with several
millions of new cases diagnosed yearly. Oral HPV infection may be associated with different
diseases of oral cavities including some cases of oropharyngeal cancer.
The aim of this report is to detect the presence of HPV DNA in samples of biopsies, oral
swabs, saliva and serum of patient with oral squamous cell carcinoma (OSCC) and controls. We
hoped to find there is correlation among the presence of HPV DNA in the several biological
materials and if it is possible to use the saliva as screening to HPV DNA detection. The
presence of tumor HPV DNA in blood may be of diagnostic and prognostic value.
This study will made at the buccal cancer center of UNESP and involved forty patients (n =
40) and forty controls. Serum samples, oral swabs and saliva will collect at the date of
diagnosis before therapy and will store at -80 ºC until analysis. Formalin-fixed
paraffin-embedded oral squamous cell carcinoma tissues and other biologic samples will
process with phenol/chloroform extraction method.
Tumors from 40 OSCC patients at the UNESP University will be obtained from biopsy with prior
consent, along with corresponding venipuncture blood, saliva collection and exfoliated buccal
cells samples. From controls will be obtained all samples except biopsy tissues. Clinical
information including tumor location, stage, and nodal status will be recorded.
Clotted blood specimens will be centrifuged at low speed for 5 min, and the serum was stored
at - 80 °C before DNA extraction. Serum samples (400 ml) will be used for DNA extraction.
Whole saliva and exfoliated buccal cells will be digested in proteinase K at 48°C during two
hours, serum and tumor tissue samples will be digested in proteinase K at 48°C overnight,
followed by phenol/chloroform extraction and ethanol precipitation of DNA for all samples.
After resuspension in 50 ml of distilled water, the mean working DNA concentrations will be
100-150 ng/ml per serum and tissues samples and 30-50 ng/ ml per whole saliva and exfoliated
buccal cells samples. For beta-globin PCR will be used 150 to 300 ng of purified total
cellular DNA, to assess the quality of the DNA using the PCR primers GH20 and PC04. After
confirmation of the presence and integrity of genomic human DNA, the same amount of DNA will
be testing for HPV DNA by nested polymerase chain reaction (PCR) in all samples. In first PCR
round degenerate consensus primers MY11 and MY09 will be using to amplify fragments of 450
bp. HPV DNA will amplified in a second round by GP5+ and GP6+ primer sets. The other reaction
components will be: 10.9 microlitres of ultra-pure water, 2.5 microlitres PCR buffer 10X, 4mM
MgCl2, 15 pmol dNTPs and 1 unit of Platinum Taq DNA polymerase. Approximately 150-300 ng of
genomic DNA from each sample will be add to the mixture. The same amount of Hela cells, with
up to 4 copies of HPV-18 per cell, will be used as positive control for HPV infection. The
negative control will be composed by all PCR components except DNA. The mixture underwent
initial denaturation to 94ºC for 10 min, before 40 PCR cycles (94ºC for 1 min; 55ºC for 1
min; 72ºC for 40) and 72°C for 4 minutes. For nPCR, two microliters of the product from the
first reaction will be used directly in a reaction containing: 0,02 mM of each primer GP5+
and GP6+(Invitrogen Life Technologies®, Brazil), which produce a 150 pb DNA fragment. The
remaining reaction components and conditions will be as described for the first round of PCR,
except for the annealing temperature that will be reduced to 43ºC. Ten microliters of the
nPCR products will be fractionated by electrophoresis in a 8% polyacrylamide gel, for 3 hours
at 100 volts. Band visualization will be performed by staining with silver nitrate solution.
Samples will be scored as either HPV DNA-positive or negative based on the inspection of
silver nitrate stained bands. PCR amplification will be performed in triplicates for each
sample. Samples will be classified as positive or negative based on gel analysis.
Differences in proportion will be evaluated by means of Fisher's exact test. A P value of
less then 0.05 will be considered statistically significant. These statistical calculations
will be performed using SPSS, version 10.0, for Windows.
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