Literature DB >> 23749641

Intravital FLIM-FRET imaging reveals dasatinib-induced spatial control of src in pancreatic cancer.

Max Nobis1, Ewan J McGhee, Jennifer P Morton, Juliane P Schwarz, Saadia A Karim, Jean Quinn, Mike Edward, Andrew D Campbell, Lynn C McGarry, T R Jeffry Evans, Valerie G Brunton, Margaret C Frame, Neil O Carragher, Yingxiao Wang, Owen J Sansom, Paul Timpson, Kurt I Anderson.   

Abstract

Cancer invasion and metastasis occur in a complex three-dimensional (3D) environment, with reciprocal feedback from the surrounding host tissue and vasculature-governing behavior. In this study, we used a novel intravital method that revealed spatiotemporal regulation of Src activity in response to the anti-invasive Src inhibitor dasatinib. A fluorescence lifetime imaging microscopy-fluorescence resonance energy transfer (FLIM-FRET) Src biosensor was used to monitor drug-targeting efficacy in a transgenic p53-mutant mouse model of pancreatic cancer. In contrast to conventional techniques, FLIM-FRET analysis allowed for accurate, time-dependent, live monitoring of drug efficacy and clearance in live tumors. In 3D organotypic cultures, we showed that a spatially distinct gradient of Src activity exists within invading tumor cells, governed by the depth of penetration into complex matrices. In parallel, this gradient was also found to exist within live tumors, where Src activity is enhanced at the invasive border relative to the tumor cortex. Upon treatment with dasatinib, we observed a switch in activity at the invasive borders, correlating with impaired metastatic capacity in vivo. Src regulation was governed by the proximity of cells to the host vasculature, as cells distal to the vasculature were regulated differentially in response to drug treatment compared with cells proximal to the vasculature. Overall, our results in live tumors revealed that a threshold of drug penetrance exists in vivo and that this can be used to map areas of poor drug-targeting efficiency within specific tumor microenvironments. We propose that using FLIM-FRET in this capacity could provide a useful preclinical tool in animal models before clinical translation. ©2013 AACR.

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Year:  2013        PMID: 23749641     DOI: 10.1158/0008-5472.CAN-12-4545

Source DB:  PubMed          Journal:  Cancer Res        ISSN: 0008-5472            Impact factor:   12.701


  46 in total

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2.  Multiphoton fluorescence lifetime imaging of chemotherapy distribution in solid tumors.

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Review 3.  Pancreatic cancer organotypics: High throughput, preclinical models for pharmacological agent evaluation.

Authors:  Stacey J Coleman; Jennifer Watt; Prabhu Arumugam; Leonardo Solaini; Elisabeta Carapuca; Mohammed Ghallab; Richard P Grose; Hemant M Kocher
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Review 4.  Developments in preclinical cancer imaging: innovating the discovery of therapeutics.

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Journal:  Nat Rev Drug Discov       Date:  2016-09-12       Impact factor: 84.694

7.  A simple approach for measuring FRET in fluorescent biosensors using two-photon microscopy.

Authors:  Richard N Day; Wen Tao; Kenneth W Dunn
Journal:  Nat Protoc       Date:  2016-09-29       Impact factor: 13.491

8.  Real-time intravital imaging of pH variation associated with osteoclast activity.

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9.  Quantitative imaging of receptor-ligand engagement in intact live animals.

Authors:  Alena Rudkouskaya; Nattawut Sinsuebphon; Jamie Ward; Kate Tubbesing; Xavier Intes; Margarida Barroso
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Review 10.  Visualizing S1P-directed cellular egress by intravital imaging.

Authors:  Christina C Giannouli; Panagiotis Chandris; Richard L Proia
Journal:  Biochim Biophys Acta       Date:  2013-10-01
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