It is well established that tumorigenesis is the result of accumulating several cooperating mutations that drive relentless proliferation and aid in metastases. Co-mutation analyses, where one oncogenic event is fixed by means of a transgene in the mouse to be infected with retrovirus, were very successful in identifying cooperating oncogenes, for example with Myc [14], or with p27Kip1 loss [19]. Without fixing any event by a transgene, viral insertional mutagenesis, though perhaps not providing all the mutations necessary for a full-blown tumor, follows the multistep scenario of tumorigenesis. Although in general the superinfection barrier largely prevents multiple proviral integrations within the same cell, re-infection does happen over time. Because it is a rare event, such cells are selected over the others only when these integrations also give a growth advantage. As a consequence, in general, most viral insertions ("co-mutations") in a single tumor are thought to be causative in its formation. With the caveats of potential passenger mutations and potential oligoclonality of tumors, co-mutation analysis may be a powerful way to find cooperating signaling pathways in tumorigenesis. For this analysis, the following two rules can be stated: (i) genes that are co-mutated in a single cancer cell represent different pathways that cooperate during carcinogenesis; and (ii) genes within the same pathway are never co-mutated. These rules assume "linear," non-branched pathways, which is a gross oversimplification. They also assume that it does not help to turn on a pathway (twice) by two integrations rather than one, but, of course, increased signal strength may indeed help tumorigenesis. For example, an obvious exception is Notch1, for which two mutations have been shown to lead to more aggressive growth than just one [35] – a fact that is reflected by our finding of three double mutants (Fig. (Fig.6;6; and unpublished), with mutations in the same two domains that are also co-mutated in patients. Nevertheless, if in a large sample set, one never finds two genes co-mutated, it seems fairly safe to assume that they are in the same pathway.

MiRNAs and low molecular weight RNAs were isolated from frozen mouse tumor tissue using the Purelink miRNA Isolation Kit (Invitrogen). The mature species of the miRNAs were measured by RT-qPCR using a stem-loop RT primer specific for each miRNA [33] in the cells listed, in triplicates. Accordingly, 50 ng of each tumor miRNA preparation was reverse transcribed with the SuperScript III First-Strand Synthesis System for RT-PCR using the following stem loop RT primers (50 nM final concentration) 5'-GTCGTATCCAGTGCAGGGTCCGAGGTATTCGCACTGGATACGACAGCACT-3'(mmu-mir-1204), 5'-GTCGTATCCAGTGCAGGGTCCGAGGTATTCGCACTGGATACGACCTCAAA-3'(mmu-mir-1205), 5'-GTCGTATCCAGTGCAGGGTCCGAGGTATTCGCACTGGATACGACACTTAA-3' (mmu-mir-1206), 5'-GTCGTATCCAGTGCAGGGTCCGAGGTATTCGCACTGGATACGACCCCTTC-3'(mmu-mir-1207-5p), 5'-GTCGTATCCAGTGCAGGGTCCGAGGTATTCGCACTGGATACGACGAGATG-3'(mmu-mir-1207-3p) and 5'-GTCGTATCCAGTGCAGGGTCCGAGGTATTCGCACTGGATACGACCCAGCC-3'(mmu-mir-1208). The reverse transcription reactions were diluted 1:5 and 5 μl of these dilutions were used in the 25 μl qPCR reactions. The annealing step was 50°C for 60s. The qPCR probes and primers were as follows: mmu-mir-1204: 5'-GCGGTGGTGGCCTGCTCT-3', 5'-GTGCAGGGTCCGAGGT-3', 5'-[56-FAM]-CACTGGATACGACAGCACTG-[36-TAMSp]-3'; mmu-mir-1205: 5'-GGCGTCTGCAGGACTGG-3', 5'-GTGCAGGGTCCGAGGT-3', 5'-[56-FAM]-CACTGGATACGACCTCAAAG-[36-TAMSp]-3', mmu-mir-1206: 5'-TTGCGGTATTCACTTGGG-3', 5'-GTGCAGGGTCCGAGGT-3', 5'-[56-FAM]-CACTGGATACGACACTTAAACA-[36-TAMSp]-3'; mmu-mir-1207-5p: 5'-TGCTGGCACGGTGGGTG-3', 5'-GTGCAGGGTCCGAGGT-3', 5'-[56-FAM]-CACTGGATACGACCCCTTCC-[36-TAMSp]-3'; mmu-mir-1207-3p: 5'-TGTCTGTCAGCTGGCCT-3', 5'-GTGCAGGGTCCGAGGT-3', 5'-[56-FAM]-CACTGGATACGACGAGATGA-[36-TAMSp]-3'; mmu-mir-1208: 5'-CCGGTCACTGTTCAGAC-3', 5'-GTGCAGGGTCCGAGGT-3', 5' [56-FAM]-CACTGGATACGACCCAGCCT-[36-TAMSp]-3'.