Sub-micromolar imaging of intrinsic chromophores by two-photon photothermal microscopy captures mitochondrial response to chemotherapy
Nathaniel Hai, Chinmayee Vallabh Prabhu Dessai, Dingcheng Sun, Jianpeng Ao, Pin-Tian Lyu, Yifan Zhu, and Ji-Xin Cheng

TL;DR
This study introduces a highly sensitive two-photon photothermal microscopy technique to detect intracellular chromophores like NADH and FAD, enabling label-free, sub-micromolar imaging of mitochondrial responses to chemotherapy.
Contribution
The paper presents a novel 2PPT microscopy method that surpasses autofluorescence limitations, allowing for specific, high-sensitivity detection of metabolic chromophores in live cells.
Findings
Achieved sub-micromolar detection limits for NADH and FAD.
Enabled differentiation of mitochondrial metabolic activity based on shape.
Studied mitochondrial metabolic changes in cancer cells during chemotherapy.
Abstract
Intracellular chromophores (e.g., NADH and FAD) play a central role in regulation of cellular metabolism. Though autofluorescence has been extensively used for label-free mapping of chromophores inside a cell, its sensitivity and molecular specificity are constrained by the low quantum yield and the fluorescence spectral overlap. Here, we address these challenges by employing a photothermal approach to measure the optical absorption of chromophores rather than its autofluorescence. By combining near-infrared pump and visible probe beams, our two-photon photothermal (2PPT) microscope exploits localized thermal transients generated through two-photon absorption, enabling detection of chromophore-specific signatures beyond the reach of autofluorescence. We demonstrate sub-micromolar limit of detection for the metabolic coenzymes NADH and FAD of 0.87 uM and 0.99 uM, respectively. Such high…
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