The early pre-mRNAs of MCV undergo

The early pre-mRNAs of MCV undergo alternative RNA splicing to
produce four mRNA isoforms: LT, sT1, sT2 and 57kT (Figure 2B). To
date, it remains unknown what RNA cis-element(s) or trans-acting
cellular factors are involved in regulating the alternative RNA splicing.
LT mRNA encodes LT antigen. Both sT1 and sT2 mRNAs encode sT,
but differ in the length of the 39 untranslated region. The 57kT mRNA
corresponds to the 17kT mRNA in SV40 and encodes a 57-kDa protein
missing a middle section of LT (Figure 2B). In contrast to SV40 sT and
MCV LT, MCV sT exhibits oncogenic activity: it transforms rodent
fibroblasts and promotes serum-independent growth of human fibroblasts.89
This is because MCV sT functions differently from SV40 sT;
MCV sT promotes eukaryotic translation initiation factor 4E-binding
protein 1 hyperphosphorylation and cap-dependent translation in a
PP2A-independent manner,89 whereas SV40 sT induces dephosphorylation
of 4E-binding protein 1 in a PP2A-dependent manner and inhibits
cap-dependent translation.91 Moreover, MCV sT suppresses the
activity of the E3 ubiqitin ligase SCFFbw7, which degrades MCV LT,
and stabilizes MCV LT through its LT-stabilization domain;92 SV40 sT
does not have an LT-stabilization domain. Although inhibition of
SCFFbw7 stabilizes MCV LT, introduction of mutations in the sT LTstabilization
domain decreases LT protein levels and eliminates synergism
in MCV DNA replication and sT-induced cell transformation.92
MCV sT is detected in 92% of MCC tissues, whereas MCV LT is only
detected in 75% of the tissues.87,89,93 However, the full function of MCV
sT in MCC cells requires other T antigens, such as LT and 57kT.