Table 3.
Overview of HPV DNA and p16INK4a studies in ESCC tissues
| Nr studies |
Author | Country | Years of diagnosis |
Biopsy type |
Genotyping method |
N (ESCC patients enrolled) |
N (ESCC valid DNA)a |
N (HPV DNA+ ESCC)(%) |
HPV types identified |
VL [viral copies per cell] |
N (HPV RNA+ among HPV DNA+) |
N (p16INK4a+ among HPV DNA+) |
N (p16INK4a+ among HPV DNA−) |
Cut off
for p16INK4a positivity |
Cross- contamination controls |
|---|---|---|---|---|---|---|---|---|---|---|---|---|---|---|---|
| InterSCOPE study | 133 | 118 | 10 (8%) | 16, 33, 35, 45, 70; 11 | 0.00 | 1 (10%) | 1 (10%) | 6 (6%) | |||||||
| South Africa | 1995–2000 | AFPE | BSGP5+6+ PCR & TS-E7-PCR | 58 | 48 | 7 (6%) | 16, 35, 45, 70; 11 | 0.00 | 1 (10%)b | 1 (10%)c | 2 (2%) | ≥25% | yes (A, B, C)d | ||
| North China (Shanxi) | 1997–2005 | FFPE | 35 | 35 | 1 (1%) | 16 | 0.00 | 0 (0%) | 0 (0%) | 3 (3%) | |||||
| Iran | 2005–2007 | FFPE | 40 | 35 | 2 (2%) | 16, 33 | 0.00 | 0 (0%) | 0 (0%) | 1 (1%) | |||||
| 1 | *Antonsson et al., 2011 | Australia | 2002–2005 | FFPE | GP5+6+ PCR + seq. | 222 | 222 | 8 (4%) | 16, 35 | nt | nt | 4 (50%)e | nte | ns | yes (A, B, C) |
| 2 | *Bellizzi et al., 2009 | USA | 1994–2007 | FFPE | ISH | 31 | 29 | 8 (4%) | none | nt | nt | 0 (0%) | 7 (24%)f | ≥25% | yes (C) |
| 3 | Cao et al., 2014 | North China (Shandong) | 2006–2008 | FFPE | ISH | 105 | 105 | 29 (28%) | 16 | nt | nt | 25 (86%) | 14 (18%) | ≥50% | nsg |
| 4 | Castillo et al., 2011 | 166 | 166 | 31 (19%) | 16, 18, 35, 45, 51, 68; 6 | 0.121 (0.05 – 0.27)h | 16 (53%)i | 42 (33%)i | |||||||
| Pakistan | 1996–2002 | FFPE | SPF1/2 InnoLiPA | 42 | 42 | 11 (26%) | 16, 18; 6 | 0.124h | nt | ns | ns | ≥10% | nsj | ||
| Columbia | 1996–2001 | 49 | 49 | 9 (18%) | 16, 18, 35, 45; 6 | 0.251h | ns | ns | |||||||
| Japan | 1987–2005 | 75 | 75 | 11 (15%) | 16, 18, 51, 68 | 0.072h | ns | ns | |||||||
| 5 | Castillo et al., 2006 | South America | 73 | 73 | 21 (29%) | 16, 18 | 12 (57%) | 25 (49%)k | |||||||
| Columbia | 1996–2001 | FFPE | GP5+6+ PCR & seq. & Southern blot | 47 | 47 | 16 (34%) | 16, 18 | nt | nt | ns | ns | ≥10% | ns | ||
| Chile | 1996–2000 | 26 | 26 | 5 (19%) | 18 | ns | ns | ||||||||
| 6 | Ding et al., 2010 | North China (Henan) | 2005–2008 | FFPE | HPV16 E6 PCR | 17 | 17 | 8 (47%) | 16 | nt | nt | 2 (25%) | 5 (56%) | ≥10% | ns |
| 7 | Doxatader et al., 2011 | USA | ns | FFPE | ISH | 20 | 20 | 1 (17%)l | ns | nt | nt | 1 (17%)l | 5 (83%)l | ≥50% | ns |
| 8 | Herbster et al., 2012 | Brazil | 2000–2009 | FFPE & DFT | GP5+6+ PCR & ISH & seq. | 264 | 264 | 34 (13%) | 16, 18, 66 | nt | nt | 7 (21%) | 3 (10%) | ns | yes (A, B, C) |
| 9 | *Koshiol et al., 2009 | North China (Linxian) | 2006–2007 | FFPE & DFT | PCR (PGMY) & SPF10 LiPA | 272 | 267 | 3 (1%) | 16, 31; 89 | nt | nt | 0 (0%) | ntm | ns | yes (A, B, C) |
| 10 | Lofdahl et al., 2012 | Sweden | 1999–2006 | FFPE | GP5+6+ PCR & Luminex | 204 | 204 | 20 (10%) | 16, 33, 45, 51, 52, 73, 82, 66; 42 | nt | nt | 4 (24%)n | 18 (16%)o | nsp | yes (C) |
| 11 | *Malik et al., 2011 | USA | 2001–2009 | FFPE | ISH | 25 | 25 | 0 (0%)q | none | nt | nt | 0 (0%)q | ntq | nsr | yes (C) |
| 12 | Shuyama et al., 2007 | China | 59 | 59 | 19 (32%) | 16, 18, 51; 6 | <0.00001 – 1.7 | 1 (5%) | 10 (25%) | ||||||
| Gansus | 1994–2005 | FFPE | SPF10 InnoLiPA & GP5+6+ PCR & Southern blot | 26 | 26 | 17 (65%) | 16 | <0.00001 | nt | nsu | 3 (12%) | ≥80% | ns | ||
| Shandogs | 33 | 33 | 2 (6%) | 16, 18 | <0.0001 – 1.7 | nsu | 7 (21%) | ||||||||
| 13 | Teng et al., 2014 | East China (Shanghai) | 1999–2011 | FFPE | PCR + RDB | 177 | 177 | 6 (3%) | 16, 35; 11 | nt | nt | 0 (0%) | 5 (3%) | ≥80% | yes (B, C) |
| 14 | *Vaiphei et al., 2013 | India | ns | DFT | PCR | 23 | 23 | 20 (87%) | 16, 18, 39, 52, 59; 6, 11 + 11 more | nt | nt | nsv | nsv | ≥40% | yes (Bw, C) |
Studies that could not be included in meta-analyses for p16INK4a due to limited tissue analyses (see specific footnotes).
Number of valid ESCC biopsy equals number of patients enrolled in each of the studies.
the single HPV16 mRNA+ case was HPV16 DNA+ by TS-E7-PCR only, did not show upregulation of p16INK4a (<10% p16INK4a+ tumor cells), and was not seropositive for HPV16 antibodies.
A single HPV DNA+/p16INK4a+ case (>75% p16INK4a+ cells) was HPV16 mRNA-. HPV DNA was identified by TS-E7-PCR only; patient was seropositive for HPV16 E6 antibodies.
Use of a new blade for sectioning of each tissue specimen (A), different laboratories for DNA extraction, PCR set up and PCR products analyses (B), use of (pretested) HPV DNA+ and HPV DNA− tissues as a control (C).
Only HPV DNA+ tumors (N=8) were tested for p16INK4a expression by IHC.
6/7 tumors were scored as 25–50%, and 1/7 tumors was scored as 50–75% p16INK4a+ tumor cells.
CSCC was used as a positive control during ISH.
Geometric mean of HPV genome copies per cell across HPV16 DNA+ tumors analyzed.
158 of 166 samples had enough material for p16INK4a analysis (30/31 HPV DNA+ and 128/135 HPV DNA− cases).
For 11 ESCC cases from Japan authors additionally analyzed tissue biopsies of tumor adjacent epithelia of which none showed HPV DNA+.
72/73 samples had enough material for p16INK4a analysis (21/21 HPV DNA+ and 51/52 HPV DNA− cases).
only p16INK4a+ cases (N=6), and the equal number of p16INK4a− cases, were tested for HPV by ISH. Only 1/6 p16INK4a+ cases was HPV DNA+.
Only HPV DNA+ ESCC were tested for p16INK4a.
17/20 HPV DNA+ ESCC had enough material for p16INK4a evaluation.
p16INK4a was evaluated in 113/184 HPV DNA− cases (6.5 HPV DNA− controls per HPV DNA+ case).
Samples were considered positive if there was homogeneous p16INK4a staining of a clear majority of tumor cells.
Only p16INK4a+ tumors (N=11) were tested for HPV DNA by ISH.
Percentage of p16INK4a+ cells was not specified. Authors stated that only biopsies with nuclear or nuclear and cytoplasmic, diffuse and strong staining were considered p16INK4a+.
Gansu is a high-incidence ESCC region in NW China and Shandong is a low-incidence ESCC region in E China.
HPV51 and HPV6 were present only as a co-infection with HPV16 in two respective cases for which region of origin was not specified.
Authors did not specify if the one p16INK4a+ case was from Gansu or from Shandong.
Number of p16INK4a+ tumors was not specified (12 tumors were positive for p16 and p63). Authors concluded that p16INK4a+ and p63 positivity did not correlate with HPV status.
Authors report using sterile forceps and blades but do not specify changing them for sectioning of each tissue sample.
Abbreviations: AFPE - alcohol-fixed paraffin-embedded, FFPE - formalin-fixed paraffin-embedded, DFT - deep frozen tissue, ISH - in situ hybridization, RDB - reverse dot blot, CSCC – cervical squamous cell carcinoma, seq. – sequencing, nt – not tested, ns - not specified