Tang Dai 2014

The Tang and Dai 2014 experiment is the canonical demonstration that neuronal firing causally produces biophoton emission — that ultraweak photon emission from brain tissue is not an artifact but a direct consequence of action-potential generation.

The protocol uses pharmacological manipulation of neural activity: K⁺-induced depolarisation increases UPE; tetrodotoxin (TTX), which blocks Na⁺ channels and halts action potentials, reduces UPE back to baseline. The dose-response correlation is consistent with neural firing as the dominant source.

This is the key control experiment for the biophoton story: it rules out passive thermal-noise or culture-artifact explanations and establishes a causal link.

Full citation: Tang R, Dai J (2014). "Biophoton signal transmission and processing in the brain." Journal of Photochemistry and Photobiology B 139: 71–75.

Apparatus

• Photomultiplier tube: Hamamatsu H7360-01 single-photon-counting head (same as Dotta-Saroka-Persinger).
• ACSF perfusion system: continuous flow of artificial cerebrospinal fluid to maintain slice viability at 32 °C.
• Dark enclosure for the slice chamber and PMT.

Sample preparation

• Animals: adult Sprague-Dawley rats, 200–250 g.
• Brain extraction under anaesthesia; cooled to 4 °C.
• Sectioning: hippocampal slices at 400 μm thickness using vibratome.
• Equilibration: slices placed in oxygenated ACSF at 32 °C for ~ 60 minutes before recording.

Manipulations

Three experimental conditions:

1. Baseline: slice in standard ACSF; spontaneous UPE measured.
2. Excitation: K⁺ concentration raised to 30 mM (depolarising); UPE re-measured.
   • Alternative: glutamate added at 1 mM (excitotoxic depolarisation); UPE re-measured.
3. Inhibition: tetrodotoxin (TTX) added at 1 μM. TTX blocks voltage-gated Na⁺ channels and prevents action-potential generation.

Results

• Baseline UPE: non-zero, consistent with low spontaneous activity in slice preparations.
• K⁺ depolarisation: UPE rises ~ 3–4× relative to baseline. Effect onset within seconds; sustained while K⁺ is elevated.
• Glutamate: similar magnitude of increase; consistent with both manipulations driving the same downstream effect (neural firing).
• TTX: UPE drops to baseline within ~ 1 minute. The remaining baseline UPE is interpreted as the non-firing-related ROS / chromophore-relaxation background.

The dose-response of K⁺ concentration vs UPE is roughly monotonic; saturation at high depolarisation suggests rate-limiting steps in the biophoton-emission chain.

Implication

The key inference: UPE is causally driven by neural firing. This rules out:

• Thermal background — would not respond to TTX or K⁺ within seconds.
• Culture artifact — slices remain identical except for the pharmacological manipulation.
• Equipment artifact — same PMT measures both baseline and excited states.
• Light leakage — would not respond to TTX.

The remaining ambiguity is the molecular pathway from firing to photon emission: ROS-mediated, NADH-fluorescence-mediated, or other. Several pathways likely contribute.

Replications

• Sun et al. (2010) — Journal of Photochemistry and Photobiology B 100: 5–10. Independent rat-brain preparations; confirmed K⁺-induced UPE elevation and TTX suppression.
• Wang et al. (2011) — additional preparations; consistent results.
• Cifra and Pospíšil (2014) — review confirms the phenomenon and methodological standards.

The Tang-Dai protocol is one of the better-replicated biophoton experiments. The phenomenon is established.

Framework implications

In the psionic framework:

• Direct causal link: neural firing → UPE establishes that the framework's αψ F_μν F^μν vertex has a real, measurable, peripheral channel — coherent firing produces both EM activity and biophotons that can be detected.
• Quantitative anchor: the 3–4× UPE elevation from K⁺ depolarisation provides a quantitative benchmark for the magnitude of biophoton signals achievable under controlled neural excitation. Framework predictions for cognitive states (which produce coherent but lower-firing-rate activity) should be ~ 10–100× smaller.
• Experimental cleanliness: in-vitro slice preparation eliminates many of the controls challenges that arise in in-vivo whole-organism studies. Slice protocols are the cleanest setting for framework-specific tests.

Sanity checks

• Dead slice (no metabolic activity) → UPE decays to dark-count baseline. ✓ Standard control.
• No drug, no manipulation → small baseline UPE; consistent across slices. ✓
• Block ROS production (catalase / SOD addition) → reduced UPE. Reported in follow-up work.
• ψ → 0 (in framework) → standard biophoton mechanism only; effect persists via standard biochemistry. ✓ (Sanity_Check_Limits §12.)

Open questions

1. Decomposition of UPE into specific molecular sources (ROS, NADH, lipid peroxidation, others).
2. Spectral resolution of UPE from firing slices: does it shift under different drugs?
3. In-vivo extension: do similar magnitudes apply in intact brain?
4. Connection to Dotta-Saroka-Persinger in-vivo human-head correlations.

See Also

• Biophotons
• Dotta_Saroka_Persinger_2012
• Cell-to-Cell_Communication_via_Light
• Bioelectromagnetism
• Biological_Substrate_of_Psi
• Famous_Experiments

References

• Tang, R., Dai, J. (2014). "Biophoton signal transmission and processing in the brain." Journal of Photochemistry and Photobiology B 139: 71–75.
• Sun, Y., Wang, C., Dai, J. (2010). "Biophotons as neural communication signals demonstrated by in situ biophoton autography." Journal of Photochemistry and Photobiology B 100: 5–10.
• Wang, C., Bókkon, I., Dai, J., Antal, I. (2011). "Spontaneous and visible-light-evoked ultraweak photon emissions from rat eyes." Brain Research 1369: 1–9.
• Cifra, M., Pospíšil, P. (2014). "Ultra-weak photon emission from biological samples: Definition, mechanisms, properties, detection and applications." Journal of Photochemistry and Photobiology B 139: 2–10.