Medical/biological study (experimental study)

Evaluating the biological effects of intermittent 1.9 GHz pulse-modulated radiofrequency fields in a series of human-derived cell lines med./bio.

By: Chauhan V, Mariampillai A, Kutzner BC, Wilkins RC, Ferrarotto C, Bellier PV, Marro L, Gajda GB, Lemay E, Thansandote A, McNamee JP

Published in: Radiat Res 2007; 167 (1): 87-93

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Aim of study (acc. to author)

To study the ability of non-thermal radiofrequency electromagnetic field exposure to affect a variety of biological processes (including apoptosis, cell cycle progression, cell viability and cytokine production) in a series of human-derived cell lines.

Background/further details

Exponentially growing cells were used and concurrent negative controls (incubator) and positive controls (heat shock for 1 h at 43°C) were included in each experiment.

Endpoint

molecular biosynthesis: cytokine production
cell viability/cell division/proliferation: cell viability, incidence of apoptosis, alterations in cell cycle progression

Exposure

- RF field
- PW pulsed wave

Exposure	Parameters
Exposure 1: 1.9 GHz Modulation type: pulsed Exposure duration: intermittent, 5 min on/10 min off, for 6 h	SAR: 1 W/kg mean (see below) SAR: 10 W/kg mean (see below)

Exposure 1

Main characteristics

Frequency	1.9 GHz
Type	electromagnetic field
Charakteristic	guided field
Polarization	circular
Exposure duration	intermittent, 5 min on/10 min off, for 6 h

Modulation

Modulation type	pulsed

Exposure setup

Exposure source	circular waveguide
Chamber	The system was allowed to equilibrate for 1 h prior to energizing the waveguides. The temperature within the cell cultures was monitored every 60 s and maintained within 37.0 ± 0.5°C for the sham, negative (incubator) control and RF-exposed samples. The samples exposed at an SAR of 10 W/kg showed cyclical fluctuations of ±0.2°C.
Setup	The 60-mm dishes containing the cell cultures in 10 ml of medium were placed atop a series of circularly polarized cylindrical waveguide applicators.
Sham exposure	A sham exposure was conducted.
Additional info	Concurrent negative and positive controls were included in each experiment. The positive (heat-shock) controls were placed on a heating block within an incubator and were maintained at 43°C for 1 h. The negative controls were placed within the same incubator but were not subjected to the heat shock.

Parameters

Measurand	Value	Type	Method	Mass	Remarks
SAR	1 W/kg	mean	estimated	-	see below
SAR	10 W/kg	mean	estimated	-	see below

Measurement and calculation details

The SAR distribution at the plane of the cells was estimated to be ±24% of the mean SAR for each RF-field treatment group, while the maximum to minimum SAR ratio within the sample region was approximately 4:1 [Gajda et al., 2002].

Reference articles

Gajda GB et al. (2002): Cylindrical waveguide applicator for in vitro exposure of cell culture samples to 1.9-GHz radiofrequency fields

Exposed system:

intact cell/cell culture
HL-60 (human acute myeloid leukaemia cells), Mono Mac 6 cells (human monocytes), TK6 cells (lymphoblastoma cells)

Methods Endpoint/measurement parameters/methodology

molecular biosynthesis: cytokine production (tumor necrosis factor alpha, interleukin 1B, interleukin 6, interleukin 8, interleukin 10, interleukin 12; cytometric bead assay, flow cytometry)
cell viability/cell division/proliferation: cell viability, incidence of apoptosis (neutral comet assay, flow cytometry), alterations in cell cycle progression (flow cytometry)

Investigated system:

isolated bio./chem. substance
intact cell/cell culture
cell supernatants

Time of investigation:

before exposure
after exposure

Main outcome of study (acc. to author)

No detectable changes in cell viability, cell cycle kinetics, incidence of apoptosis, or cytokine expression were found in any of radiofrequency exposed groups in any of the cell lines tested in comparison to the sham exposed controls. However, the positive control samples displayed a significant decrease in cell viability, increase in apoptosis, and alteration in cell cycle kinetics.

Study character:

medical/biological study
experimental study
full/main study

Study funded by

Health Canada

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