Alessandro Zunino scite author profile

To date, the feasibility of super-resolution microscopy for imaging live and thick samples is still limited. Stimulated emission depletion (STED) microscopy requires high-intensity illumination to achieve sub-diffraction resolution, potentially introducing photodamage to live specimens. Moreover, the out-of-focus background may degrade the signal stemming from the focal plane. Here, we propose a new method to mitigate these limitations without drawbacks. First, we enhance a STED microscope with a detector array, enabling image scanning microscopy (ISM). Therefore, we implement STED-ISM, a method that exploits the working principle of ISM to reduce the depletion intensity and achieve a target resolution. Later, we develop Focus-ISM, a strategy to improve the optical sectioning and remove the background of any ISM-based imaging technique, with or without a STED beam. The proposed approach requires minimal architectural changes to a conventional microscope but provides substantial advantages for live and thick sample imaging.

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Acousto-optic systems for advanced microscopy

Duocastella

Surdo

Zunino

et al. 2020

J. Phys. Photonics

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Acoustic waves in an optical medium cause rapid periodic changes in the refraction index, leading to diffraction effects. Such acoustically controlled diffraction can be used to modulate, deflect, and focus light at microsecond timescales, paving the way for advanced optical microscopy designs that feature unprecedented spatiotemporal resolution. In this article, we review the operational principles, optical properties, and recent applications of acousto-optic (AO) systems for advanced microscopy, including random-access scanning, ultrafast confocal and multiphoton imaging, and fast inertia-free light-sheet microscopy. As AO technology is reaching maturity, designing new microscope architectures that utilize AO elements is more attractive than ever, providing new exciting opportunities in fields as impactful as optical metrology, neuroscience, embryogenesis, and high-content screening.

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GM1 Ganglioside role in the interaction of Alpha-synuclein with lipid membranes: Morphology and structure

Perissinotto

Rondelli

Parisse

et al. 2019

Biophysical Chemistry

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Alpha-Synuclein (AS) is the protein playing the major role in Parkinson's disease (PD), a neurological disorder characterized by the degeneration of dopaminergic neurons and the accumulation of AS into amyloid plaques. The aggregation of AS into intermediate aggregates, called oligomers, and their pathological relation with biological membranes are considered key steps in the development and progression of the disease. Here we propose a multi-technique approach to study the effects of AS in its monomeric and oligomeric forms on artificial lipid membranes containing GM1 ganglioside. GM1 is a component of functional membrane micro-domains, called lipid rafts, and has been demonstrated to bind AS in neurons. With the aim to understand the relation between gangliosides and AS, here we exploit the complementarity of microscopy (Atomic Force Microscopy) and neutron scattering (Small Angle Neutron Scattering and Neutron Reflectometry) techniques to analyze the structural changes of two different membranes (Phosphatidylcholine and Phosphatidylcholine/GM1) upon binding with AS. We observe the monomer-and oligomer-interactions are both limited to the external membrane leaflet and that the presence of ganglioside leads to a stronger interaction of the membranes and AS in its monomeric and oligomeric forms with a stronger aggressiveness in the latter. These results support the hypothesis of the critical role of lipid rafts not only in the biofunctioning of the protein, but even in the development and the progression of the Parkinson's disease. and SANS-YS instruments of the Budapest Neutron Center. High purity functionalization of the Si block surface by the staff of the BioMEMS group of Inst. Tech. Physics and Mater.

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Dynamic Multifocus Laser Writing with Acousto‐Optofluidics

Zunino

Surdo

2019

Adv Materials Technologies

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Laser writing of materials is normally performed by the sequential scanning of a single focused beam across a sample. This process is time‐consuming and it can severely limit the throughput of laser systems in key applications such as surgery, microelectronics, or manufacturing. A parallelization strategy based on ultrasound waves in a liquid to diffract light into multiple beamlets is reported. Adjusting amplitude, frequency, or phase of ultrasound allows tunable multifocus distributions with sub‐microsecond control. When combined with sample translation, the dynamic splitting of light leads to high‐throughput laser processing, as demonstrated by locally modifying the morphological and wettability properties of metals, polymers, and ceramics. The results illustrate how acousto‐optofluidic systems are universal tools for fast multifocus generation, with potential impact in fields such as imaging or optical trapping.

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