Michael S. Roberts, Yousuf H. Mohammed, Astrid Magenau, James R.W. Conway, Jennifer P. Morton, Sean C. Warren, Paul Timpson, Douglas Strathdee, David Herrmann, Yingxiao Wang, Thomas R. Cox, Pauline Mélénec, Heidi C.E. Welch, Tri Giang Phan, Imogen Moran, Max Nobis, Kurt I. Anderson, Claire Vennin, Warren, Sean C, Nobis, Max, Magenau, Astrid, Mohammed, Yousuf H, Herrmann, David, Moran, Imogen, Vennin, Claire, Conway, James RW, Melenec, Pauline, Cox, Thomas R, Wang, Yingxiao, Morton, Jennifer P, Welch, Heidi CE, Strathdee, Douglas, Anderson, Kurt I, Phan, Tri Giang, Roberts, Michael S, Timpson, Paul, Warren, Sean C [0000-0002-5253-7147], Nobis, Max [0000-0002-1861-1390], Herrmann, David [0000-0002-9514-7501], Cox, Thomas R [0000-0001-9294-1745], Wang, Yingxiao [0000-0003-0265-326X], Strathdee, Douglas [0000-0003-2959-4327], Anderson, Kurt I [0000-0002-9324-9598], Phan, Tri Giang [0000-0002-4909-2984], and Apollo - University of Cambridge Repository
Intravital microscopy can provide unique insights into the function of biological processes in a native context. However, physiological motion caused by peristalsis, respiration and the heartbeat can present a significant challenge, particularly for functional readouts such as fluorescence lifetime imaging (FLIM), which require longer acquisition times to obtain a quantitative readout. Here, we present and benchmark Galene, a versatile multi-platform software tool for image-based correction of sample motion blurring in both time resolved and conventional laser scanning fluorescence microscopy data in two and three dimensions. We show that Galene is able to resolve intravital FLIM-FRET images of intra-abdominal organs in murine models and NADH autofluorescence of human dermal tissue imaging subject to a wide range of physiological motions. Thus, Galene can enable FLIM imaging in situations where a stable imaging platform is not always possible and rescue previously discarded quantitative imaging data., eLife digest Understanding how molecules and cells behave in living animals can give researchers key insights into what goes wrong in diseases such as cancer, and how well potential treatments for these diseases work. A number of tools help us to see these processes. For example, fluorescent ‘biosensors’ change colour to tell us how active a particular protein is. This can indicate how well a drug works in different parts of a tumour. High resolution microscopy makes it possible to image events happening in single cells, or even specific parts of a cell. However, small movements like those due to the heartbeat or breathing can blur the images, making it difficult to study living animals. This is particularly problematic for images that take several minutes to capture. Warren et al. have now developed a new open source software tool called Galene. The tool can correct for small movements in images collected by a technique called fluorescence lifetime imaging microscopy (FLIM). As a result, clear images can be captured in situations that were not previously possible. For example, Warren et al. watched cancer cells migrating to the liver of a mouse from the spleen over 24 hours, and, using a fluorescent biosensor, showed that a repurposed drug interferes with how well the cells can attach to the liver. In addition, Warren et al. used the software to take steady 3D images of human skin in a volunteer’s arm, which could be used to study drug penetration. Galene could help researchers to study a wide range of biological processes in living animals. The software can also be applied to existing data to clean up blurred images. In the future Galene could be further developed to work with the imaging techniques used during surgery. For example, surgeons could use it to help them find the edges of tumours.