4.8 Article

Quantum-enhanced nonlinear microscopy

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NATURE
卷 594, 期 7862, 页码 201-+

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NATURE RESEARCH
DOI: 10.1038/s41586-021-03528-w

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A quantum microscope utilizing quantum photon correlations achieves a signal-to-noise ratio beyond the photodamage limit of conventional microscopy, improving imaging precision and resolution of biological structures within cells. Coherent Raman microscopes, incorporating bright quantum correlated illumination, offer subwavelength resolution and enhanced concentration sensitivity, enabling observation of previously unresolved biological structures. Overcoming the photodamage limit allows for significant improvements in signal-to-noise ratio and imaging speed.
A quantum microscope obtains signal-to-noise beyond the photodamage limits of conventional microscopy, revealing biological structures within cells that would not otherwise be resolved. The performance of light microscopes is limited by the stochastic nature of light, which exists in discrete packets of energy known as photons. Randomness in the times that photons are detected introduces shot noise, which fundamentally constrains sensitivity, resolution and speed(1). Although the long-established solution to this problem is to increase the intensity of the illumination light, this is not always possible when investigating living systems, because bright lasers can severely disturb biological processes(2-4). Theory predicts that biological imaging may be improved without increasing light intensity by using quantum photon correlations(1,5). Here we experimentally show that quantum correlations allow a signal-to-noise ratio beyond the photodamage limit of conventional microscopy. Our microscope is a coherent Raman microscope that offers subwavelength resolution and incorporates bright quantum correlated illumination. The correlations allow imaging of molecular bonds within a cell with a 35 per cent improved signal-to-noise ratio compared with conventional microscopy, corresponding to a 14 per cent improvement in concentration sensitivity. This enables the observation of biological structures that would not otherwise be resolved. Coherent Raman microscopes allow highly selective biomolecular fingerprinting in unlabelled specimens(6,7), but photodamage is a major roadblock for many applications(8,9). By showing that the photodamage limit can be overcome, our work will enable order-of-magnitude improvements in the signal-to-noise ratio and the imaging speed.

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