CELLFOOD® - A
Beneficial Colloid?
Report of an Investigation into the Colloidal Nature
of CELLFOOD
Author
Dr. David Fairhurst,
PhD
Background
CELLFOOD is a highly
concentrated proprietary liquid formulation comprising a host of trace elements,
minerals, enzymes, amino-acids, solvated (dissolved) oxygen and deuterated
hydrogen. It is sold as a complete mineral and nutritional supplement to enhance
the biochemical activities and functions of the body.
It has been
suggested (1), based on the anatomy and composition of the CELLFOOD, that it may
be a colloidal suspension functioning in a manner similar to, and compatible
with, body fluids (such as blood, lymph, cerebrospinal, synovial and bone). The
purpose of the present study is to determine the colloidal nature or behavior,
if any, of CELLFOOD. The various mechanisms by which CELLFOOD may act, as a
nutritional supplement, is beyond the scope of this report.
Introduction
It is, perhaps, instructive, to first define
exactly what constitutes "the colloidal state" and why such systems - colloids -
are so important.
The overwhelming majority of manufactured products,
that we deal with on a day-to-day basis involve, either in the final state or at
some stage of their production, suspensions of particulate materials, emulsion
droplets or air bubbles dispersed often at high volume fraction. Any suspension
may exist in three distinct conditions depending upon the degree of subdivision
of the discontinuous (internal) phase. For example, during the hydraulic
transport of a coarsely ground limestone/water slurry through a pipeline, we can
determine the technologically important physical properties of the system from
the bulk properties of the separate phases and also by application of
appropriate laws of mechanics and hydraulics; the chemical composition of the
phases, as such, is unimportant. If, however, the same limestone-water mixture
is subjected to grinding to reduce the particle size to below one micrometer
(10-6m), the system takes on characteristics unpredicted by the laws that
previously applied. The suspension may behave as a semi-solid paste or as a
free-flowing liquid depending, now, upon the presence of trace amounts of
certain dissolved electrolytes that have no discernable effect on the original
mixture. Further reduction of particle size to atomic/molecular dimensions, (say
by dissolving with hydrochloric acid) will yield a system with behavior
characteristic of liquid phases, i.e. a solution.
It is the intermediate
systems - termed colloidal dispersions - that are of special interest because of
their unique properties. But first, how, then, do we define the colloidal-size
range? As a very rough guide, colloidal-sized particles lie within the range of
one or two nanometers (10-9m) to a few micrometers, i.e. from about the size of
lactoglobulin to about the size of a small bacterium (such as staphylococcus).
The red blood cell is about seven micrometers in diameter and is treated as a
colloidal dispersion (2) and has long been used as a calibration reference
material (3). Hence, while the lower size limit, at which we differentiate
between a colloidal particle and a dissolved molecule, is understandably vague;
the upper size limit is annoyingly arbitrary!
The colloidal domain,
therefore, forms a critical interface between micro- and macroscopic regimes; it
has been termed "the place where physics, chemistry, biology and technology
meet" (4). The essential character common to every colloidal system is the large
area-to-volume ratio for the particles involved (5). This can result in
exceptional catalytic activity and chemical/biochemical reactivity; it directly
impacts biomedical processes in, for example, controlled release of drugs after
digestion, inhalation etc. The efficacy of such systems is dependent on the
actual particle size distribution (PSD) of the particles and the chemical
composition of the suspending fluid (6); this determines whether or not the
particles will adsorb at, or permeate, a cell membrane (a phopholipid bilayer).
From this it can be readily appreciated that not every colloidal system is
"beneficial". For example, natural water contains dissolved organic carbon
(DOC), arising from the microbial and photolytic degradation of natural organic
matter (NOM), creating, in effect, organic pollutants in the form of a colloidal
dispersion. Current water treatment processes can remove only about 50% of NOM -
a cause for concern by the World Health Organization. On a positive note, in
recent times, the advent of "nanotechnology" has created excitement in a wide
array of sectors in the scientific, medical and financial communities. Yet
nanoscale materials are, by definition, colloidal systems.
Sample Preparation and Measurement
When any material
is dispersed in a fluid, the properties of the resultant suspension are
dependent upon two fundamental parameters, namely:
(i) The extent of the
particle-fluid interface. This is characterized by properties such as the
particle size/particle size distribution and particle shape and porosity,
and
(ii) The particle-fluid interfacial chemistry. This is
characterized by the type and the degree of dissociation of any material surface
functional groups in relation to the fluid chemical composition
There are
many parameters that can be measured which reflect the extent of the interface
and the interfacial chemistry. Two reliable and well-established parameters are,
respectively, particle size and zeta potential; the techniques, that have been
devised to determine them, are extremely diverse (7-9). The present study
utilized an instrument based on dynamic light scattering for particle size
measurement and phase analysis light scattering (10) for determination of the
zeta potential. All measurements were conducted by Mr.William Bernt (Particle
Characterization Laboratories, Novato, CA) using a ZetaPALS instrument with the
Particle Sizing Option (Brookhaven Instruments Corporation, NY).
Particle
Size Analysis: The CELLFOOD concentrate was diluted using DI (VWR 18Mohm) water
that had been filtered through a 0.1 m filter. The instrument was validated
using a 92nm (+/- 3.7nm) PS latex suspension (NIST traceable) obtained from Duke
Scientific, CA). The filtered DI water was also measured as a
blank.
Zeta Potential Analysis: The CELLFOOD concentrate was
measured as received and also diluted using DI (VWR 18Mohm) water. The
instrument was validated using an NIST electrophoresis reference (SRM 1980) of
2.53 +/- 0.12 mobility units (equivalent to a zeta potential of 32.4 +/- 1.5
mV).
Results and Discussion
The particle
size results of the instrument validation and test sample are given in the Bernt
(PCL) Report of May 14, 2001. The filtered DI water produced random scatter in
the correlation function and a count rate too low for any analysis, consistent
with the absence of any particles in the water. For the validation sample, it is
clear from all methods of analysis of the raw data (Cumulants, NNLS and CONTIN)
that the instrument passes validation. The particle size distribution (PSD) is
clearly a narrow unimodal as shown by the polydispersity index of <0.01. The
overall average particle size (PS), from all data, was calculated to be 91.2nm,
well within specification.
Colloidal systems are generally,
however, of a polydisperse nature, i.e. the particles in a particular sample
vary in size and CELLFOOD is no exception. The method of cumulants gives an
average PS of 2.45 m and the polydispersity index of 0.322 suggests a very broad
PSD. This was confirmed by the NNLS and CONTIN analysis and, in addition, both
algorithms resulted in a bimodal distribution with modal sizes at approximately
1.48 m and 6.63 m. Such a PSD is entirely consistent with the extremely complex
compositional nature of CELLFOOD and the shape would, of necessity, impart
unusual performance characteristics.
The zeta potential results of
the instrument validation and test samples are given in the Bernt (PCL) Reports
of May 15, 2001 and February 23, 2002. The filtered DI water had a measured
conductance of 9 S, as might be expected and, since the particle size analysis
did not detect any particles it is also not surprising that the measured zeta
potential was close to zero (0.03mV). The instrument passed validation: the
(average) measured conductance of the electrophoresis reference suspension was
1469 S and an average calculated zeta potential of 32.1mV - both values within
specification.
The first test sample was the CELLFOOD concentrate run
without dilution. The measured conductance was an amazing 200,000 S, undoubtedly
due to the very high concentration of electrolytes in the composition. The zeta
potential was calculated to be -22.7mV, consistent with the fact that, under
normal circumstances, biological cells tend to carry a net negative surface
charge (or zeta potential). For example red blood cells suspended in isotonic
saline solution (essentially 0.145 molar NaCl) have a measured zeta potential of
approximately -14mV. Typically, micro-organisms have zeta potentials in the
range of -5 to -15 mV. Now, the magnitude of the zeta potential always
"decreases" (i.e., in this case, becomes less negative) with increase in
electrolyte concentration. The conductance of the CELLFOOD concentrate is
however, considerably larger than that for isotonic saline and yet the zeta
potential is more negative. This is very unusual and it suggests that the
colloidal particles in CELLFOOD may possess very special properties that could
influence metabolic changes or alterations in blood flow properties and increase
absorption of components from body fluids. It is well accepted that the
magnitude and sign of the charge on a biological surface will influence its
interaction with other surfaces or molecules.
The second test
sample was the CELLFOOD concentrate diluted into filtered DI water at the rate
of 8 drops to 8oz identical with the recommended daily dosage. As expected, the
conductance now decreased to around 3500 S. However, the zeta potential hardly
changed. Indeed, it decreased slightly to -20 mV, when it should have increased
(i.e. become more negative). It is not possible, at this time, to speculate on
why this should occur because the composition of the CELLFOOD is so complex.
However, such behavior while desirable, is very unusual.
It is known that
glacial waters contain mineral colloidal particles and a virtual "soup" of
dissolved salts (electrolytes) and that drinking such water has a very positive
benefit on the health and longevity of the users. In addition, it has been
reported that the use of such waters in industrial formulations (such as cement)
seems to dramatically improve performance characteristics. A detailed analysis
of the surface and interfacial properties of glacial waters was able to
substantiate some of the claims (11) even though the mechanisms involved could
not be identified. Although it has not been possible to carry out a similar
in-depth analysis of CELLFOOD, the similarities in colloidal nature lead this
author to conclude that CELLFOOD is indeed, a very beneficial
colloid.
Conclusion
CELLFOOD is clearly
colloidal dispersion. The shape of the particle size distribution and the
magnitude of the zeta potential would suggest that the product would be
compatible with body fluids. The data supports the notion that CELLFOOD should
be beneficial as a nutritional supplement.
References
1. D.S. Dyer,
"CellFood®: Vital Cellular Nutrition for the New Millenium", Feedback Books,
(2000).
2. G.V.F. Seaman, "The Red Blood Cell", Academic Press, (1975).
3.
D.V. Richmond and D.J. Fisher, in "Advances in Microbial Physiology",
(1973).
4. D.F. Evans and H. Wennerström, "The Colloidal Domain", VCH
Publishers, (1994).
5. D.H.Everett, Basic Principles of Colloid Science,
Royal Society of Chemistry Publications, (1988).
6. R.J. Hunter,
"Introduction to Modern Colloid Science", Oxford University Press,
(1993).
7. T.Allen, "Particle Size Analysis Measurement", Chapman &
Hall, (1993)
8. D.J.Shaw, "Electrophorsesis", Academic Press, (1969).
9.
P.McFadyen and D. Fairhurst, in "Nanoceramics" (ed. R.Freer), British Ceramic
Society, (1993)
10. W.W. Tscharnuter and D. Fairhurst,, ACS Symposium
Series
11. B. Marlow and D. Fairhurst, unpublished results/ Univ. Mass.
Internal report