Single-cell Raman and fluorescence microscopy reveal the association of lipid bodies with phagosomes in leukocytes

Manen, Henk‐Jan van; Kraan, Yvonne M.; Roos, Dirk; Otto, Cees

doi:10.1073/pnas.0502746102

Cited by 288 publications

(265 citation statements)

References 47 publications

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“…In addition to the above associations, LDs make a kiss-and-run type contact with phagosomes (van Manen et al 2005). This transient encounter in neutrophils was speculated to supply phagosomes with arachidonic acid for NADPH oxidase activation.…”

Section: Lipid Droplets In the Cellular Context Interactions With Othmentioning

confidence: 99%

Not Just Fat: The Structure and Function of the Lipid Droplet

Fujimoto

Parton²

2011

Cold Spring Harbor Perspectives in Biology

401

336

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Lipid droplets (LDs) are independent organelles that are composed of a lipid ester core and a surface phospholipid monolayer. Recent studies have revealed many new proteins, functions, and phenomena associated with LDs. In addition, a number of diseases related to LDs are beginning to be understood at the molecular level. It is now clear that LDs are not an inert store of excess lipids but are dynamically engaged in various cellular functions, some of which are not directly related to lipid metabolism. Compared to conventional membrane organelles, there are still many uncertainties concerning the molecular architecture of LDs and how each function is placed in a structural context. Recent findings and remaining questions are discussed.

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Section: Lipid Droplets In the Cellular Context Interactions With Othmentioning

confidence: 99%

Not Just Fat: The Structure and Function of the Lipid Droplet

Fujimoto

Parton²

2011

Cold Spring Harbor Perspectives in Biology

401

336

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“…Due to the specificity of the drug spectral signature, the released drug can be identified. As few as few thousand drug molecules can be detected by this methodology [103].…”

Section: High Resolution Confocal Raman Imaging Of Individual Cellsmentioning

confidence: 99%

Molecular pathology via IR and Raman spectral imaging

Diem¹,

Mazur²,

Lenau³

et al. 2013

Journal of Biophotonics

175

115

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Journal of BIOPHOTONICSDuring the last 15 years, vibrational spectroscopic methods have been developed that can be viewed as molecular pathology methods that depend on sampling the entire genome, proteome and metabolome of cells and tissues, rather than probing for the presence of selected markers. First, this review introduces the background and fundamentals of the spectroscopies underlying the new methodologies, namely infrared and Raman spectroscopy. Then, results are presented in the context of spectral histopathology of tissues for detection of metastases in lymph nodes, squamous cell carcinoma, adenocarcinomas, brain tumors and brain metastases. Results from spectral cytopathology of cells are discussed for screening of oral and cervical mucosa, and circulating tumor cells. It is concluded that infrared and Raman spectroscopy can complement histopathology and reveal information that is available in classical methods only by costly and time-consuming steps such as immunohistochemistry, polymerase chain reaction or gene arrays. Due to the inherent sensitivity toward changes in the bio-molecular composition of different cell and tissue types, vibrational spectroscopy can even provide information that is in some cases superior to that of any one of the conventional techniques.Schematic of spectral histopathology (SHP) process: diagnostic algorithm is developed by spectral data of well documented specimens and subsequently applied to unknown dataset.

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“…Liposome Uptake into Cells-Apart from imaging subcellular features, as discussed in the previous sections, Raman imaging may provide an opportunity to follow the uptake of molecules into cells. One way to distinguish incorporated molecules inside cells is to use deuterated compounds (van Manen et al, 2005). C-D stretching vibrations are shifted away from those of C-H groups by a factor of about the square root of the masses of H and D, or about a factor of 1.4.…”

Section: Label Free Imaging Of Cellular Mitochondrial Distribution-thismentioning

confidence: 99%

Chapter 10 Infrared and Raman Microscopy in Cell Biology

Matthäus

Bird

Miljković

et al. 2008

Methods in Cell Biology

163

119

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This chapter presents novel microscopic methods to monitor cell biological processes of live or fixed cells without the use of any dye, stains, or other contrast agent. These methods are based on spectral techniques that detect inherent spectroscopic properties of biochemical constituents of cells, or parts thereof. Two different modalities have been developed for this task. One of them is infrared micro-spectroscopy, in which an average snapshot of a cell's biochemical composition is collected at a spatial resolution of typically 25 mm. This technique, which is extremely sensitive and can collect such a snapshot in fractions of a second, is particularly suited for studying gross biochemical changes. The other technique, Raman microscopy (also known as Raman microspectroscopy), is ideally suited to study variations of cellular composition on the scale of subcellular organelles, since its spatial resolution is as good as that of fluorescence microscopy. Both techniques exhibit the fingerprint sensitivity of vibrational spectroscopy toward biochemical composition, and can be used to follow a variety of cellular processes.

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Single-cell Raman and fluorescence microscopy reveal the association of lipid bodies with phagosomes in leukocytes

Cited by 288 publications

References 47 publications

Not Just Fat: The Structure and Function of the Lipid Droplet

Not Just Fat: The Structure and Function of the Lipid Droplet

Molecular pathology via IR and Raman spectral imaging

Chapter 10 Infrared and Raman Microscopy in Cell Biology

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