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Dive into the research topics where Aleem Syed is active.

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Featured researches published by Aleem Syed.


Journal of the American Chemical Society | 2015

BODIPY-Derived Photoremovable Protecting Groups Unmasked with Green Light

Pratik P. Goswami; Aleem Syed; Christie L. Beck; Toshia R. Albright; Kaitlyn M. Mahoney; Ryan Unash; Emily A. Smith; Arthur H. Winter

Photoremovable protecting groups derived from meso-substituted BODIPY dyes release acetic acid with green wavelengths >500 nm. Photorelease is demonstrated in cultured S2 cells. The photocaging structures were identified by our previously proposed strategy of computationally searching for carbocations with low-energy diradical states as a possible indicator of a nearby productive conical intersection. The superior optical properties of these photocages make them promising alternatives to the popular o-nitrobenzyl photocage systems.


Photochemistry and Photobiology | 2014

The number of accumulated photons and the quality of stimulated emission depletion lifetime images

Aleem Syed; Michael David Lesoine; Ujjal Bhattacharjee; Jacob W. Petrich; Emily A. Smith

Time binning is used to increase the number of photon counts in the peak channel of stimulated emission depletion fluorescence lifetime decay curves to determine how it affects the resulting lifetime image. The fluorescence lifetime of the fluorophore, Alexa Fluor 594 phalloidin, bound to F‐actin is probed in cultured S2 cells at a spatial resolution of ~40 nm. This corresponds to a 10‐fold smaller probe volume compared to confocal imaging, and a reduced number of photons contributing to the signal. Pixel‐by‐pixel fluorescence lifetime measurements and error analysis show that an average of 40 ± 30 photon counts in the peak channel with a signal‐to‐noise ratio of 20 is enough to calculate a reliable fluorescence lifetime from a single exponential fluorescence decay. No heterogeneity in the actin cytoskeleton in different regions of the cultured cells was measured in the 40–400 nm spatial regime.


Reviews in Analytical Chemistry | 2017

Raman Imaging in Cell Membranes, Lipid-Rich Organelles, and Lipid Bilayers

Aleem Syed; Emily A. Smith

Raman-based optical imaging is a promising analytical tool for noninvasive, label-free chemical imaging of lipid bilayers and cellular membranes. Imaging using spontaneous Raman scattering suffers from a low intensity that hinders its use in some cellular applications. However, developments in coherent Raman imaging, surface-enhanced Raman imaging, and tip-enhanced Raman imaging have enabled video-rate imaging, excellent detection limits, and nanometer spatial resolution, respectively. After a brief introduction to these commonly used Raman imaging techniques for cell membrane studies, this review discusses selected applications of these modalities for chemical imaging of membrane proteins and lipids. Finally, recent developments in chemical tags for Raman imaging and their applications in the analysis of selected cell membrane components are summarized. Ongoing developments toward improving the temporal and spatial resolution of Raman imaging and small-molecule tags with strong Raman scattering cross sections continue to expand the utility of Raman imaging for diverse cell membrane studies.


Journal of the American Chemical Society | 2018

Family of BODIPY Photocages Cleaved by Single Photons of Visible/Near-Infrared Light

Julie A. Peterson; Chamari Wijesooriya; Elizabeth J. Gehrmann; Kaitlyn M. Mahoney; Pratik P. Goswami; Toshia R. Albright; Aleem Syed; Andrew S. Dutton; Emily A. Smith; Arthur H. Winter

Photocages are light-sensitive chemical protecting groups that provide external control over when, where, and how much of a biological substrate is activated in cells using targeted light irradiation. Regrettably, most popular photocages (e.g., o-nitrobenzyl groups) absorb cell-damaging ultraviolet wavelengths. A challenge with achieving longer wavelength bond-breaking photochemistry is that long-wavelength-absorbing chromophores have shorter excited-state lifetimes and diminished excited-state energies. However, here we report the synthesis of a family of BODIPY-derived photocages with tunable absorptions across the visible/near-infrared that release chemical cargo under irradiation. Derivatives with appended styryl groups feature absorptions above 700 nm, yielding photocages cleaved with the highest known wavelengths of light via a direct single-photon-release mechanism. Photorelease with red light is demonstrated in living HeLa cells, Drosophila S2 cells, and bovine GM07373 cells upon ∼5 min irradiation. No cytotoxicity is observed at 20 μM photocage concentration using the trypan blue exclusion assay. Improved B-alkylated derivatives feature improved quantum efficiencies of photorelease ∼20-fold larger, on par with the popular o-nitrobenzyl photocages (εΦ = 50-100 M-1 cm-1), but absorbing red/near-IR light in the biological window instead of UV light.


Journal of Organic Chemistry | 2014

Self-immolative phthalate esters sensitive to hydrogen peroxide and light

Kaitlyn M. Mahoney; Pratik P. Goswami; Aleem Syed; Patrick Kolker; Brian Shannan; Emily A. Smith; Arthur H. Winter

Self-immolative aryl phthalate esters were conjugated with cleavable masking groups sensitive to light and hydrogen peroxide. The phthalate linker releases the fluorescent dye 7-hydroxycoumarin upon exposure to light or H2O2, respectively, leading to an increase in fluorescence. The light-sensitive aryl phthalate ester is demonstrated as a pro-fluorophore in cultured S2 cells.


Biochimica et Biophysica Acta | 2016

Ligand binding affinity and changes in the lateral diffusion of receptor for advanced glycation endproducts (RAGE)

Aleem Syed; Qiaochu Zhu; Emily A. Smith

The effect of ligand on the lateral diffusion of receptor for advanced glycation endproducts (RAGE), a receptor involved in numerous pathological conditions, remains unknown. Single particle tracking experiments that use quantum dots specifically bound to hemagglutinin (HA)-tagged RAGE (HA-RAGE) are reported to elucidate the effect of ligand binding on HA-RAGE diffusion in GM07373 cell membranes. The ligand used in these studies is methylglyoxal modified-bovine serum albumin (MGO-BSA) containing advanced glycation end products modifications. The binding affinity between soluble RAGE and MGO-BSA increases by 1.8 to 9.7-fold as the percent primary amine modification increases from 24 to 74% and with increasing negative charge on the MGO-BSA. Ligand incubation affects the HA-RAGE diffusion coefficient, the radius of confinement, and duration of confinement. There is, however, no correlation between MGO-BSA ligand binding affinity with soluble RAGE and the extent of the changes in HA-RAGE lateral diffusion. The ligand induced changes to HA-RAGE lateral diffusion do not occur when cholesterol is depleted from the cell membrane, indicating the mechanism for ligand-induced changes to HA-RAGE diffusion is cholesterol dependent. The results presented here serve as a first step in unraveling how ligand influences RAGE lateral diffusion.


Physical Biology | 2014

Single particle tracking with sterol modulation reveals the cholesterol-mediated diffusion properties of integrin receptors

Neha Arora; Aleem Syed; Suzanne Sander; Emily A. Smith


European Biophysics Journal | 2018

Lateral diffusion and signaling of receptor for advanced glycation end-products (RAGE): a receptor involved in chronic inflammation

Aleem Syed; Qiaochu Zhu; Emily A. Smith


European Biophysics Journal | 2014

Role of insulin receptor and insulin signaling on αPS2CβPS integrins’ lateral diffusion

Dipak Mainali; Aleem Syed; Neha Arora; Emily A. Smith


Biophysical Journal | 2012

Extracellular, Membrane and Intracellular Proteins that Alter Integrin Cell Membrane Diffusion and Clustering

Emily A. Smith; Neha Arora; Dipak Mainali; Aleem Syed

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Emily A. Smith

United States Department of Energy

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