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Differential mRNA expression of Ara-C-metabolizing enzymes explains Ara-C sensitivity in MLL gene-rearranged infant acute lymphoblastic leukemia

Authors :
Stam, R.W. (Ronald)
Boer, M.L. (Monique) den
Meijerink, J.P.P. (Jules)
Ebus, M.E.
Peters, G.J. (Godefridus)
Noordhuis, P.
Janka-Schaub, G.E. (Gritta)
Armstrong, S.A. (Scott)
Korsmeyer, S.J.
Pieters, R. (Rob)
Stam, R.W. (Ronald)
Boer, M.L. (Monique) den
Meijerink, J.P.P. (Jules)
Ebus, M.E.
Peters, G.J. (Godefridus)
Noordhuis, P.
Janka-Schaub, G.E. (Gritta)
Armstrong, S.A. (Scott)
Korsmeyer, S.J.
Pieters, R. (Rob)
Publication Year :
2003

Abstract

Infant acute lymphoblastic leukemia (ALL) is characterized by a high incidence of mixed lineage leukemia (MLL) gene rearrangements, a poor outcome, and resistance to chemotherapeutic drugs. One exception is cytosine arabinoside (Ara-C), to which infant ALL cells are highly sensitive. To investigate the mechanism underlying Ara-C sensitivity in infants with ALL, mRNA levels of Ara-C-metabolizing enzymes were measured in infants (n = 18) and older children (noninfants) with ALL (n = 24). In the present study, infant ALL cells were 3.3-fold more sensitive to Ara-C (P =.007) and accumulated 2.3-fold more Ara-CTP (P =.011) upon exposure to Ara-C, compared with older children with ALL. Real-time quantitative reverse trancriptase-polymerase chain reaction (RT-PCR) (TaqMan) revealed that infants express 2-fold less of the Ara-C phosphorylating enzyme deoxycytidine kinase (dCK) mRNA (P =.026) but 2.5-fold more mRNA of the equilibrative nucleoside transporter 1 (hENT1), responsible for Ara-C membrane transport (P =.001). The mRNA expression of pyrimidine nucleotidase I (PN-I), cytidine deaminase (CDA), and deoxycytidylate deaminase (dCMPD) did not differ significantly between both groups. hENT1 mRNA expression inversely correlated with in vitro resistance to Ara-C (r(s) = -0.58, P =.006). The same differences concerning dCK and hENT1 mRNA expression were observed

Details

Database :
OAIster
Notes :
application/pdf, Blood, English
Publication Type :
Electronic Resource
Accession number :
edsoai.ocn929973560
Document Type :
Electronic Resource