Copy number of the Adenomatous Polyposis Coli gene is not always neutral in sporadic colorectal cancers with loss of heterozygosity for the gene

All tissue specimens were formalin-fixed and paraffin-embedded. Histological slides stained with H&E were examined and the areas of relevant tissue were identified and marked, as was an area of normal tissue. Consecutive unstained slides were prepared from the paraffin blocks and the corresponding areas were isolated with a blade under a dissecting microscope and transferred to an eppendorf tube. The paraffin wax was removed with xylene and ethanol washes. The cellular material was lysed in a proteinase K buffer solution. DNA was isolated and purified using the Qiagen QIAamp DNA Mini Kit (Qiagen Inc., Valencia, CA). DNA concentration was determined using a NanoDrop ND-1000 spectrophotometer (NanoDrop Technologies, Wilmington DE).

All microsatellite primer sets were ordered through the Life Technologies Custom Oligo Synthesis Service (genomicorders@lifetech.com). In all primer sets the forward primer contained a 5′ fluorescent label while the reverse primer contained a 5′- GTGTCTT tail. All PCR reactions were performed in 30 μl volumes using 100 ng of template with Applied Biosystems reagents (Roche Molecular Systems, Inc., Branchburg, NJ) and a final 1.5 mM MgCl₂ concentration. Reactions were run on an ABI 9700 thermal cycler (Applied Biosystems, Foster City, CA) under the following conditions: 5 min denaturation at 94 °C, followed by 35 cycles of a 30 s denaturation at 94 °C, 30 s annealing at 55 °C, and a 60 s elongation at 72 °C, with a final 30 min extension at 72 °C. PCR products were separated by capillary electrophoresis with an ABI 3130 Genetic Analyzer and the data was processed with GeneMapper software v4.0 (Applied Biosystems, Foster City, CA).

Loss of heterozygosity of the APC gene was determined by amplification of the CA repeat region within the D5S346 loci. PCR of microsatellites is a standard method for determining LOH. D5S346 demonstrates linkage disequilibrium with APC and is thus a well suited marker. The primer sequences used were: 5′-ACT CAC TCT AGT GAT AAA TCG GG-3′ (forward) and 5′-AGC AGA TAA GAC AAG TAT TAC TAG TT-3′ (reverse). Samples that were homozygous using the D5S346 primer set were analyzed using repeats within the D5S1965 or D5S492 loci. LOH of the DCC gene was determined by amplification of the CA repeat marker D18S1407 with the primers 5′-TTC CCT TCA TTT CAC TGG GA-3′ (forward) and 5′-CTA GAT GGA TGT GAC TTG GC-3′ (reverse). Samples that were homozygous using the D18S1407 primer set were analyzed using repeats within the D18S58 or D18S61 loci. For all LOH studies, neoplastic tissue was evaluated simultaneously with normal colonic mucosal tissue from the same patient.

The primers used for LOH analysis all contain polymorphic CA repeats that usually generate two distinct PCR allele products (maternal and paternal). However, if the alleles are the same molecular weight, then they coincide. That particular CA repeat is considered homozygous and the primer set is uninformative for that sample. If the alleles are of different molecular weights, then the ratio of the allele peak heights is used to determine LOH. We define the allele ratio as the height of the higher molecular weight PCR product to the lower molecular weigh PCR product. In normal tissue, the lower molecular weight allele PCR product is always greater in height than the higher molecular weight product due to normal PCR bias (Fig. 3). Therefore, to determine LOH, the ratio of the band intensities (peak heights) of the two alleles in the neoplastic tissue is divided by the corresponding ratio in the normal mucosa. This ratio of ratios normalizes for this intrinsic PCR amplification bias, as well as for any inter-run variations in absolute peak heights. Resultant ratios of tumor to normal tissues that approach 1 are considered to have no LOH. We define a tumor to have LOH if the resultant ratio is less than 0.5 or greater than 2.0, depending on whether the higher or lower molecular weight allele is lost, respectively. This is a conservative value, but one that insures true LOH [22]. Approximately 40 % of the 530 colorectal cancers we have studied demonstrated LOH of the APC gene by our criteria. We selected 38 cases with sufficient available DNA and with an APC allele ratio below 0.5, with an average of 0.32 and a range from 0.12 to 0.49 (Table 1).

Microsatellite instability (MSI) was detected using the Bethesda panel of markers that includes two mononucleotide markers: BAT25 and BAT26, and three dinucleotide markers: D2S123, D5S346, and D17S250. A 1997 National Cancer Institute workshop recommended a ‘reference panel’ of 5 microsatellite markers for the detection of MSI in colorectal cancer [23]. This panel continues to be a useful screen for MSI. For all MSI studies neoplastic tissue was evaluated simultaneously with normal colonic mucosal tissue from the same patient. Microsatellite instability for a given primer set was defined as a change in the allele pattern, with the appearance of one or more new PCR products relative to those produced by the normal DNA. A tumor was defined as MSI-high if two or more of the five markers had a changed allele pattern, and is referred to as “MSI”. Since all tumors were microsatellite stable, we concluded that the MSI pathway was not a part of the molecular profile in these cases, and we did not assay for methylation.

We used Sanger sequencing for detecting KRAS gene point mutations. Sanger sequencing is the gold standard for determining point mutations. The codon 12/13 region in exon 2 of the KRAS oncogene was amplified using the primer set 5′-AAGGCCTGCTGAAAATGACTG-3′ and 5′-GGTCCTGCACCAGTAATATGCA-3′. Hot-start PCR was performed in 50 μl volumes with AmpliTaq Gold polymerase and ABI reagents using 100 ng of template DNA, 50 pmols of primer, and 2.0 mM MgCl₂ on a GeneAmp PCR System 9700 (Applied Biosystems, Foster City, CA). PCR consisted of an initial 8 min denaturation at 94 °C, followed by 40 total cycles of a 30 s denaturation at 94 °C, a 30 s annealing, and a one minute elongation at 72 °C, with a final 30 min extension at 72 °C. The annealing temperature was stepped down at 62, 60 and 58 °C for 5, 20, and 15 cycles, respectively.

The copy number status of the APC gene was ascertained using multiplex ligation-dependent probe amplification [24]. We employed the SALSA® MLPA® P043-B1 APC Kit according to the manufacturer’s instructions (MRC-Holland, Amsterdam, The Netherlands). We used this method because the MLPA method allows amplification of multiple PCR targets with a small amount of DNA harvested from paraffin blocks.

This kit uses 26 probes spanning the APC gene and additional 13 reference probes. Tumor and normal DNA from paraffin-embedded tissue was analyzed as sample and reference runs, respectively. Two hundred nanograms of genomic DNA were hybridized with the probe mixture followed by a ligation reaction. All of the probes contain universal PCR primer recognition sites, and only ligated probes were subsequently PCR amplified. A single PCR reaction therefore amplified all 39 ligation products. PCR reactions were analyzed on an ABI 3130 Genetic Analyzer with GeneMapper v4.0 software. GeneMapper data were subsequently exported for copy number analysis using Coffalyser v9.4 software available at the MRC-Holland website (www.​mlpa.​com).

Within the Coffalyser software, the “Tumor Analysis Least Squares (LS)” analysis option was chosen to normalize and analyze the MLPA data. This method normalizes (intra-sample) the APC probe peak areas versus the reference probes areas for all sample runs, and then normalizes (inter-sample) each tumor specimen run versus the normal DNA reference runs. The ratios of the changes in the APC probe areas from the tumor DNA verses the normal reference DNA are reported. The Coffalyser analysis assigns ratio values less than 0.7 as having a copy number loss, greater than 1.3 as a having a copy number gain, and ratio values between 0.7 and 1.3 as normal for each APC probe [25]. This assay does not determine exact number of copies of APC, rather it provides information relative to normal tissue and to the internal control.

For any given tumor sample, we assigned overall copy number loss or gain if 2/3 (rounded to the nearest whole number) or more of the 26 APC probes had ratio values consistently <0.7 or >1.3, respectively. If 1/3 (rounded to the nearest whole number) or less or the 26 APC probes showed a loss or gain we assigned the sample as copy number neutral. If 1/3 to 2/3 of the probes showed a consistent loss or gain we assigned the sample as having a partial copy number loss or gain.