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Conversion Efficiencies of a Few Living Microbial Cells Detected at a High Throughput by Droplet-Based ESI-MS

机译:通过基于液滴的ESI-MS在高吞吐量中检测到几种生命微生物细胞的转化效率

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The label-free and sensitive detection of synthesis products from single microbial cells remains the bottleneck for determining the specific turnover numbers of individual whole-cell biocatalysts. We demonstrate the detection of lysine synthesized by only a few living cells in microfluidic droplets via mass spectrometry. Biocatalyst turnover numbers were analyzed using rationally designed reaction environments compatible with mass spectrometry, which were decoupled from cell growth and showed high specific turnover rates (similar to 1 fmol/(cell h)), high conversion yields ( 25%), and long-term catalyst stability (>14h). The heterogeneity of the cellular reactivity of only 15 +/- 5 single biocatalysts per droplet could be demonstrated for the first time by parallelizing the droplet incubation. These results enable the resolution of biocatalysis beyond averages of populations. This is a key step toward quantifying specific reactivities of single cells as minimal functional catalytic units.
机译:单个微生物细胞的合成产物的无标记和敏感性检测仍然是确定各种细胞生物催化剂的特定周转数的瓶颈。我们证明了通过质谱法通过微流体液滴中仅在微流体液滴中仅通过质谱来合成的赖氨酸。使用理性设计的反应环境与质谱法分析的生物催化剂营业额与细胞生长分离并显示出高特异性周转率(类似于1 fmol /(细胞H)),高转化率(25%)和长 - 术语催化剂稳定性(> 14h)。通过并使液滴孵育并使液滴相平时,首次证明每滴15 +/- 5个单一生物催化剂的细胞反应性的异质性。这些结果使得能够超出人口平均值的生物催化。这是定量单细胞的特异性反应性作为最小官能催化单元的关键步骤。

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