根除绿豆芽中的超弱光子发射

IF 3.261
Alasdair M. Mackenzie , Holly E. Smith , Rhys R. Mould , Jimmy D. Bell , Alistair V.W. Nunn , Stanley W. Botchway
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引用次数: 0

摘要

众所周知,生命已经进化到能够利用和产生光,例如光合作用、视觉和生物发光。鲜为人知的是,在正常代谢过程中,它可以产生1-100个光子s−1 cm-2,称为超弱光子发射(UPE),生物光子发射或生物自发光。这些代谢光子的最高产生似乎发生在氧化应激期间,由于活性氧(ROS)的产生和衰变,以及它们与细胞其他成分的相互作用。为了进一步研究这一点,我们配置了一个灵敏的检测系统来研究绿豆萌发过程中的光子发射。在这里,我们研究了在21±1°C的恒定温度下,在一个光密箱中生长绿豆7天,使用双顶和底对置光电倍增管。在这段时间内,我们发现从种子中生长出来的绿豆平均产生5±1个计数,比背景高5−1。随着新豆茎的生长,它们的排放量逐渐线性增加,最高可达30±1计数s−1,与先前的文献一致。除了这种“稳态”发光外,我们还观察到延迟发光和干旱胁迫响应发光,这是以前在其他物种中观察到的。最后,我们还观察到在样品下检测到的持续约3小时的2到15个计数s−1的偶发性增加的排放事件,并将其归因于次生根的生长。然后,我们用生长激素过氧化氢(H2O2, 167µM)或3-吲哚乙酸(IAA, 0.5µM)的水溶液浇水诱导次生根的形成。两种激素均在稳态以上表现出长时间的辐射增加,在3-5天内,与单独浇水相比,形成的次生根数至少增加了3倍。我们还观察到H2O2的光子发射峰值显著增加(474和1738 cps,而水单独为28和55 cps),我们将其归因于直接ROS反应发射,并通过对死亡植物的测量证实了这一点。总的来说,我们已经扩展并展示了一种仪器和生物系统,可以可靠地产生和测量内在代谢光子,这是亚历山大·古维奇在100年前首次观察到的。
本文章由计算机程序翻译,如有差异,请以英文原文为准。

Rooting out ultraweak photon emission a-mung bean sprouts

Rooting out ultraweak photon emission a-mung bean sprouts

Rooting out ultraweak photon emission a-mung bean sprouts

It is well known that life has evolved to use and generate light, for instance, photosynthesis, vision and bioluminescence. What is less well known is that during normal metabolism, it can generate 1–100 photons s−1 cm–2 known as ultra-weak photon emission (UPE), biophoton emission or biological autoluminescence. The highest generation of these metabolic photons seem to occur during oxidative stress due to the generation and decay of reactive oxygen species (ROS), and their interaction with other components of the cell. To study this further, we have configured a sensitive detection system to study photon emission in germinating mung beans.

Here we investigated growing mung beans over 7 days at a constant temperature of 21 ± 1 °C in a light tight box, using dual top and bottom opposing photomultiplier tubes. Over this time period we showed that in total, mung beans grown from seeds generated an average of 5 ± 1 counts s−1 above background. As the new bean stems grew, they showed a gradual linear increase in emission of up to 30 ± 1 counts s−1, in agreement with previous literature. In addition to this “steady-state” emission we also observe delayed luminescence and drought-stress response emission previously observed in other species. Finally, we also observe episodic increased emission events of between 2 and 15 counts s−1 for durations of around 3 h detected underneath the sample, and assign these to the growing of secondary roots.

We then induce secondary root formation using aqueous solutions of growth hormones hydrogen peroxide (H2O2, 167 µM) or 3-indole acetic acid (IAA, 0.5 µM) for watering. Both hormones show prolonged increase in emission above steady-state, over days 3–5 with at least 3 times the number of secondary roots formed compared with water alone. We also observed a significant peak increase in photon emission (474 and 1738 cps vs. 28 and 55 cps for water alone) for the H2O2 which we attribute to direct ROS reaction emission as confirmed by measurement on dead plants.

Altogether we have expanded upon and demonstrated an instrument and biological system for reliably producing and measuring intrinsic metabolic photons, first observed 100 years ago by Alexander Gurwitsch.

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