PT  - JOURNAL ARTICLE
AU  - S Nisar
AU  - M Birch
AU  - K Rankin
TI  - G204(P) Osteosarcoma cell culture on collagen surfaces and in hypoxia alters mmp expression
AID  - 10.1136/archdischild-2015-308599.198
DP  - 2015 Apr 01
TA  - Archives of Disease in Childhood
PG  - A87--A87
VI  - 100
IP  - Suppl 3
4099  - http://adc.bmj.com/content/100/Suppl_3/A87.2.short
4100  - http://adc.bmj.com/content/100/Suppl_3/A87.2.full
SO  - Arch Dis Child2015 Apr 01; 100
AB  - Osteosarcoma is the most common primary malignant bone tumour in children. The survival rate has not improved much over the last 25 years, and therefore there is a lot to learn about the pathogenesis of this cancer. The interactions of tumour cells with their environment and hypoxia have been identified as key drivers of tumour growth and metastasis. Matrix-metallo proteinases (MMPs) are involved in this process. MMPs are zinc-endopeptidases that are able to degrade the extra-cellular matrix and are over-expressed in many tumours. Membrane-type (MT1)-MMP and MMP-2 expression is positively associated with tumour progression in a range of tumours, but their role is not well characterised in osteosarcoma. Two osteosarcoma cell lines were cultured on culture plastic or collagen surfaces in either normoxia or hypoxia. Proliferation was assessed using the SRB assay which showed osteosarcoma cells proliferate slightly slower in hypoxia. Immunofluorescence microscopy was employed to visualise MT1-MMP – this revealed MT1-MMP packaging and localisation was altered in hypoxia and there was formation of invadopodia on collagen. Gelatinase expression, assessed using zymography of supernatants, demonstrated increased proMMP-2 activation by cells cultured on collagen, particularly by U2OS cells. Cell lysates were probed for MT1-MMP using western blotting. ELISA of the culture supernatant was used to measure TIMP-2 expression. Less active MT1-MMP was detected in the lysates of the U2OS cells which coincided with a decreased amount of TIMP-2 detected in the supernatant. This study contributes to our understanding of the activation of MMPs and the possible role of MT1-MMP in this regard.