Compensation of loss of protein function in microsatellite-unstable colon cancer cells (HCT116): A gene-dependent effect on the cell surface glycan profile

doi:10.1093/glycob/cwp040

Glycobiology Advance Access originally published online on March 17, 2009
Glycobiology 2009 19(7):726-734; doi:10.1093/glycob/cwp040

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Compensation of loss of protein function in microsatellite-unstable colon cancer cells (HCT116): A gene-dependent effect on the cell surface glycan profile

Georgios Patsos^2,3, Sabine André³, Nina Roeckel², Roland Gromes², Johannes Gebert², Jürgen Kopitz¹^,2 and Hans-Joachim Gabius³

² Department of Applied Tumor Biology, Institute of Pathology, University Hospital Heidelberg, D-69120 Heidelberg
³ Institute of Physiological Chemistry, Faculty of Veterinary Medicine, Ludwig-Maximilians-University Munich, D-80539 Munich, Germany

¹ To whom correspondence should be addressed: Tel: +49-6221-562683; Fax: +49-6221-562683; e-mail: juergen.kopitz{at}med.uni-heidelberg.de

Received on November 25, 2008; revised on January 30, 2009; accepted on March 12, 2009

Tumors that display a high level of microsatellite instability(MSI-H) accumulate somatic frameshift mutations in several genes.The compensation of this loss of function by transfection representsa suitable approach to tie respective gene deficiency to alterationsin cellular characteristics. In view of the emerging significanceof cell surface glycans as biochemical signals for presentation/activityof various receptors/integrins and for susceptibility to adhesion/growth-regulatorytissue lectins, we examined the glycophenotype in the MSI-Hcolon cancer cell line HCT116 for activin type 2 receptor (ACVR2),absent in melanoma 2 (AIM2), and transforming growth factorβ-type 2 receptor (TGFBR2) known to be associated withMSI colorectal carcinogenesis. A panel of probes specific forfunctional carbohydrate epitopes including human lectins wasused to trace changes in cell surface levels, thereby initiatingglycan analysis related to MSI. In particular, the presenceof core substitutions and branching in N-glycans, the sialylationstatus of N- and O-glycans, and the presence of Le^a/x-epitopeswere profiled. Transient transfection affected the glycophenotype,depending on the nature of the gene and the probe. The TGFBR2presence reduced binding of probes specific for a core substitutionand increased branch length in N-glycosylation, even reachinga P-value of 0.0016. ACVR2/AIM2 influenced core 1 mucin-typeO-glycosylation differentially, upregulation by ACVR2, and downregulationby AIM2. These alterations of cell surface glycosylation bygene products that are not directly associated with the machineryfor glycan generation direct attention to pursue analysis ofglycosylation in MSI tumor cells on the level of target glycoproteinsand open the way for functional studies.

Key words: carcinogenesis / glycosylation / lectins / malignancy / microsatellite

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