| Solution to the Puzzle
of Human Cardiovascular Disease: Its Primary Cause Is Ascorbate
Deficiency, Leading to the Deposition of Lipoprotein(a) and Fibrinogen/Fibrin
in the Vascular Wall (1991)
Rath M, Pauling L. Journal of Orthomolecular Medicine,
6:125-134.
Summary
Human cardiovascular disease (CVD) is the
result of the accumulation of lipoprotein(a), Lp(a), rather than
of low density lipoprotein (LDL), in the vascular wall. It is
generally not the consequence of plasma LDL levels, but rather
of the level of Lp(a), which is formed in the liver in amounts
largely determined by the rate of synthesis of apo(a). This rate
is increased by low ascorbate concentrations. Human CVD is primarily
a degenerative disease caused by ascorbate deficiency. This deficiency
is the result of the inability of humans to synthesize endogenous
ascorbate combined with an insufficient dietary ascorbate intake.
The deficiency is aggravated by genetic defects such as the LDL
receptor defect and by exogenous risk factors for CVD leading
to additional ascorbate depletion. Ascorbate deficiency results
in morphologic changes of the vascular wall. In order to avoid
the fatal consequences of extreme ascorbate depletion, such as
hemorrhagic bleeding in scurvy, ascorbate deficiency simultaneously
increases the plasma concentration of vasoconstrictive and hemostatic
risk factors, including Lp(a) and fibrinogen. Chronic ascorbate
deficiency leads to the extracellular accumulation of Lp(a) and
fibrinogen/fibrin, the hallmarks of the atherosclerotic lesion.
The underlying impairment of the vessel wall is unmasked mainly
at sites of altered hemodynamic conditions, leading to myocardial
infarction and stroke as the predominant manifestations of human
CVD. Thus for patients with coronary or cerebrovascular disease
the instability of the vessel wall due to ascorbate deficiency
is the leading risk factor, rather than plasma constituents. In
contrast, risk factors in plasma trigger the manifestation of
peripheral vascular disease (PVD). In this condition plasma constituent
such as oxygen free radicals from cigarette smoke or oxidatively
modified triglyceride-rich lipoproteins exert a noxious effect
on the vascular wall in the periphery and PVD develops. Ascorbate
depletion of the vascular tissue is also a precondition for the
manifestation of PVD. Human CVD is multifactorial. Ascorbate deficiency,
however, is the common denominator of this disease. The comprehensive
pathogenetic and therapeutic concept presented in this paper represents
the solution to the puzzle of human cardiovascular disease and
should lead to the improvement of human health
Full Study
My dear Kepler, what do you say of the leading philosophers here
to whom I have offered a thousand times of my own accord to show
my studies, but who, with the lazy obstinacy of a serpent who
has eaten his fill, have never consented to look at the planets,
or moon, or telescope? Verily, just as serpents close their eyes,
so do men close their eyes to the light of truth."
Galileo Galilei in a letter
to Johannes Kepler ca. 1630
Introduction
We recently formulated the concept that lipoprotein(a), Lp(a),
is a surrogate for ascorbate, vitamin C. (1) This concept revealed
the physiological role of Lp(a) as well as new therapeutic approaches.
On the basis of earlier work and additional experimental and clinical
evidence we now present a detailed theory of human CVD. The primary
cause of human CVD is a deficiency in ascorbate leading to the
deposition of Lp(a) and fibrinogen/fibrin in the vascular wall.
We elucidate the interaction of ascorbate and Lp(a) and present
a pathomechanism that differs from existing concepts (2,3,4) in
that it is able to explain the unique features of human atherosclerosis.
We also present prophylactic and therapeutic considerations that
open new pathways to prevention and treatment of CVD.
The Pivotal Role of Lp(a)
in Human Cardiovascular Disease
Lp(a) was discovered by Kare Berg in 1963. (5) It is closely similar
to LDL, the main difference being that a glycoprotein, apo(a),
is attached by a disulfide bond to the apoprotein of LDL, apo
B, giving a larger surface area to the lipoprotein sphere. The
c-DNA sequence of apo(a) shows a striking homology to that of
plasminogen (6), with multiple repeats of kringle 4, one kringle
5 and a protesase domain. Because of the homology of apo(a) with
plasminogen Lp(a) has been called the missing link between atherogenesis
and thrombogenesis (7).
Evidence that Lp(a), not LDL, is the primary lipoprotein
responsible for initiating the development of atherosclerosis
was reported by one of us and his colleagues at Hamburg University
(8,9,10). In the most comprehensive studies assessing the role
of Lp(a) in human vascular wall yet reported it was found that
Lp(a), not LDL accumulates selectively in the vascular wall of
CVD patients. Moreover the extracellular accumulation of Lp(a)
was closely correlated to the development of atherosclerotic plaques.
Most importantly, in several hundreds of histological
cross sections from the human coronary arteries and the aorta
immunostaining for apoB, without congruent staining for apo(a)
was a rare event, indicating that the vascular wall deposition
of LDL alone occurs rarely (9). The deposition of Lp(a) in the
vascular wall as determined by immuno-morphometric analysis because
extraction methods overestimate the role of LDL: a major fraction
of Lp(a) is found dissociated in the vascular wall into apo(a)
and the LSDL-like particle particularly under post-mortem conditions.
(8) Earlier investigators have evidently failed to differentiate
between LDL and Lp(a) so that the initiation of atherosclerotic
lesions was incorrectly attributed to LDL.
This conclusion was recently confirmed by a study
determining plasma risk factors in patients with inherited LDL-receptor
defects. In these familial hypercholesterolemic patients the incidence
of CVD was significantly determined by the Lp(a) plasma concentration,
with total cholesterol and LDL cholesterol in plasma not related
to the clinical manifestation of CVD.
There is now strong clinical and experimental evidence
that Lp(a) is a more important risk factor than total cholesterol
or LDL-cholesterol for coronary heart disease (12), stroke (13),
as well as restenosis of vein grafts after coronary bypass surgery
(14). We therefore conclude that Lp(a) is the lipoprotein primarily
responsible for the initiation of human CVD. The role of LDL is
best characterized as an aggravating risk factor for CVD in patients
with simultaneously elevated Lp(a) plasma levels.
The Ascorbate-Lp(a) Connection
We observed that Lp(a) has mainly been detected in the plasma
of man, other primates and a few other species that have lost
the ability to synthesize ascorbate and consequently have low
ascorbate levels compared to animals with endogenous ascorbate
production. We do not exclude, however, that small amounts of
Lp(a) will also be found in other species. The loss of ascorbate
synthesis is the result of a genetic mutation in the gene for
L-gulono-c -lactone oxidase; this mutation occurred 40 million
years ago in an ancestor of the primates. Subsequently, Lp(a)
became a major plasma constituent in primates and man. We therefore
proposed that Lp(a) is a surrogate for ascorbate. Vice versa,
ascorbate is a surrogate for Lp(a), since in most species Lp(a)
is replaced by ascorbate without any disadvantage.
Previously, it has been assumed that Lp(a) is primarily
a pathogenic particle and that Lp(a) plasma concentrations are
primarily determined by genetic factors. Our publication of the
Lp(a)-ascorbate connection marked a turning point in research
directions and suggested numerous investigations. Subsequently,
it was shown that ascorbate, the strongest reducing agent normally
present in the body, and also synthetic reducing agents such as
N-acetylcysteine (15), decrease Lp(a) plasma levels. In a clinical
trial in CVD patients an increased intake of ascorbate lowered
the plasma Lp(a) level (unpublished observations).
Moreover, we proposed that Lp(a) strengthens the
vascular wall, particularly in ascorbate deficiency. At low ascorbate
concentrations the synthesis of collagen and elastin is impaired
and the deposition of Lp(a) helps to control the resulting instability
of the vessel wall and to contain disease progression. Apo(a),
a macromolecule, would compensate for this impairment and its
demonstrated binding to glycosaminoglycans and other compounds
of the extracellular matrix would be beneficial. Moreover, apo(a)
has been shown top bind with high affinity to proline and hydroxyproline
and is likely to bind to collagen and elastin, macromolecules
that are enriched in these amino acid residues. Increased intake
of ascorbate eliminates the need for Lp(a) to strengthen the blood
vessels and thus ascorbate can replace Lp(a).
We have recently been able to confirm that ascorbate
can replace Lp(a) at the site of the disease process. In this
pilot study we used the hypoascorbemic guinea pig , an animal
like man, unable to synthesize ascorbate but able to synthesize
apo(a). When fed dietary ascorbate in small amounts, corresponding
approximately to the usual human intake, these animals rapidly
develop atherosclerotic plaques and deposit Lp(a) in the vascular
wall. Larger intakes of ascorbate inhibited the deposition of
Lp(a) in the arterial wall and prevented the development of atherosclerosis.
(16)
Ascorbate and the Regulation
of Plasma Lp(a)
Lp(a) plasma levels among individuals vary by as much as
1000 fold. This considerable variation is to a large extent the
result of genetic factors determining the synthesis of apo(a),
but also those of apoB and lipids. It may be that the modifying
genes controlling apo(a) synthesis at the optimum level have not
yet become fully effective, so that in some individuals this synthesis
has overshot the mark, predisposing them to CVD.
Beside genetic factors, Lp(a) plasma concentrations
are also regulated by dietary factors, one of them being niacin,
which has been shown to lower plasma Lp(a) levels (17). Another
dietary factor is ascorbate. We have obtained preliminary results
that ascorbate decreases apo(a) synthesis in human hepatoma cells
in vitro. Ascorbate may also decrease the assembly of the Lp(a)
particle by reducing the disulfide formation between apo(a) and
apo B in the liver.
Ascorbate Defiency, the
Risk Profile for CVD and Lp(a)
Ascorbate depletion is the common metabolic denominator
of endogenous and exogenous risk factors for CVD. Many genetic
defects are associated with ascorbate deficiency. As a result
of a genetic defect the rate-constants of certain enzyme-controlled
metabolic reactions are decreased. These rate constants can be
increased towards normal values by increasing the concentrations
of certain cofactors (18). In the attempt to normalize these decreased
rate constants, ascorbate and other essential cofactors for metabolic
reactions are depleted. Ascorbate, a potent reducing and hydroxylating
molecule, is destroyed in these reactions. Accordingly, in the
effort to control the damage done by the genetic defect the level
of ascorbate is decreased, exacerbating the general deleterious
effects of ascorbate deficiency.
One of the genetic defects where the ascorbate
depleting steps are well characterized is the LDL receptor defect.
All the expressions of LDL receptors (19) the inhibition of 3-hydroxy-3-methyl-glutaryl
coenzyme A reductase in the synthesis of cholesterol (20), the
protection of LDL against oxidative modification (21) and the
stimulation of 7a -hydroxylase in the catabolism of cholesterol
to bile acids (22). We suggest that it is ascorbate deficiency
that is the real cause of the premature CVD associated with this
inherited disease, exacerbated by the genetic defect.
In this context the recent study in familial hypercholesterolemic
patients by Seed et al. (11) is of interest. In this study elevated
LDL or the underlying genetic defect of the LDL-receptor were
not correlated with CVD. Thus this genetic defect leading to ascorbate
deficiency in combination with the genetic deposition for high
Lp(a) levels significantly increased the risk of premature CVD.
As do genetic defects, exogenous risk factors for
CVD lead to ascorbate depletion. The observed correlation between
a high fat diet or cigarette smoking and CVD can also be explained
as the result of induced ascorbate deficiency, caused by destruction
of ascorbate in the catabolism of lipids and the effort to detoxify
the substances in the smoke. With insufficient dietary ascorbate
resupplementation, both endogenous and exogenous risk factors
for CVD aggravate ascorbate deficiency and accelerate CVD development.
Ascorbate Deficiency and
the Vascular Wall
Ascorbemia, the total depletion of ascorbate in scurvy,
leads to a complete loss of the integrity and stability of the
vascular wall and to the extravasation of blood into the perivascular
area. Hypoascorbemia, leads to early forms of this impairment.
The vascular endothelium is directly affected by
ascorbate deficiency. Characteristic features are changes in the
cellular morphology and the presence of large intercellular gaps.
These changes lead to the loss of the function of the endothelium
as a barrier between the blood and the vascular wall, to increased
permeability, and consequently to increased infiltration of plasma
constituents into the vascular wall.
The extracellular matrix of the wall is affected.
Collagen and elastin, the principal macromolecules of this matrix,
are made from their precursors, procollagen, and proelastin, by
hydroxylation of prolyl and lysyl residues. Ascorbate deficiency
leads to an incomplete hydroxylation and thus weakens the extracellular
matrix. Alterations of the endothelium and loose connective tissue
are known to be characteristic features of atherosclerotic plaques.
To limit the fatal consequences of prolonged ascorbate
deficiency metabolic counter measures were developed under strong
evolutionary pressure.
Ascorbate Deficiency and
Metabolic Countermeasurs
To limit the consequences of prolonged ascorbate deficiency
metabolic countermeasures were developed under strong evolutionary
pressure. The most detrimental effect of ascorbate depletion is
blood loss. Thus ascorbate deficiency, to prevent the extravasation
of blood, triggers a whole series of metabolic reactions, with
the primary aim of inducing vasoconstriction and hemostasis.
It is therefore not surprising that ascorbate deficiency
induces virtually all the risk factors predisposing to atherogenesis
and thrombogenesis, most of them with immediate clinical significance.
In the first line of defense against the danger of perivascular
bleeding increased levels of thromboxane and decreased levels
of prostacyclin (23) and prostaglandin E lead to vasoconstriction
and hemostasis. We have shown that prolonged ascorbate deficiency
increases fibrinogen and Lp(a) plasma levels and in this situation
the antifibrinolyitic properties of Lp(a) become beneficial.
We are aware that there is no one-to-one relation
between ascorbate and Lp(a). Lp(a) is a rather late part in a
sequence of acute-phase reactants, or risk factors induced by
ascorbate deficiency. Because of its lipid deposition in the vascular
wall, however, Lp(a) is particularly detrimental.
The therapeutic implications are evident: ascorbate
supplementation increases the levels of prostacyclin and potentially
EDRF, the endothelial derived relaxing factor. This potent vasodilative
factor is identical with nitric oxide and ascorbate may preserve
the active form of EDRF by inhibiting oxidation to nitrogen dioxide.
Simultaneously, ascorbate decreases the levels of thromboxane,
fibrinogen, and Lp(a) and thereby contributes to a fundamental
improvement of the risk profile in clinical cardiology.
The Roles of Lp(a) and
Fibrinogen in the Vascular Wall
In the Hamburg studies Lp(a) was found mainly deposited
together with fibrinogen/fibrin (10). Moreover, Lp(a) has been
shown to bind to immobilized fibrinogen/fibrin (25) and evidence
for a direct binding of Lp(a) to fibrinogen/fibrin in the vascular
wall was reported (9). All these observations can now be explained.
In ascorbate deficiency the need for increased plasma concentrations
of Lp(a) and fibrinogen, for binding of Lp(a) to fibrinogen/ fibrin
in the vascular wall, and for its selective retention become evident.
The hemostatic properties of Lp(a) and fibrinogen
are needed to counteract the deleterious consequences of ascorbate
deficiency. Lp(a) also has functions in the containment of diseases
and the repair of tissues. Free-radical-induced and plasmin-induced
tissue degradation are established pathways.
We have suggested that apo(a), because of many
disulfide groups that can be reduced by ascorbate to thiols, can
itself function as an antioxidant (1). Moreover, we now suggest
that because of its homology to plasmin Lp(a) also inhibits plasmin-induced
tissue degradation. The lipid content of the Lp(a) particle simultaneously
provides the substrate for cell repair. In order to exert its
physiological functions Lp(a) is deposited as an intact lipoprotein
particle and can be isolated from the vascular wall (8). The extracellular
accumulation of Lp(a) in the vascular wall is an independent pathomechanism
of human CVD which is at variance with concepts suggesting the
cellular uptake and degradation of lipoproteins by scavenger cells
is a prerequisite for atherogenesis (2,4).
A Theory for Human Cardiovascular
Disease
We are now able to present a novel pathomechanism for human
cardiovascular disease. This disease is primarily a degenerative
disease caused by chronic ascorbate deficiency. The extracellular
deposition of Lp(a) and fibrinogen is a defense mechanism to limit
the damage done by this deficiency. Under chronic conditions this
defense may, however, turn into a pathologic process leading to
the continued accumulation of Lp(a) and fibrinogen/fibrin in the
vascular wall. Thus Lp(a) and fibrinogen/fibrin become the hallmarks
of the atherosclerotic lesion (see figure).
Figure a.
The impairment of the integrity of the vascular
wall in ascorbate deficiency leads to increased infiltration of
plasma constituents and to intimal thickening throughout the vascular
system but not necessarily to the development of atherosclerotic
plaques. If, however, altered hemodynamic conditions reveal the
underlying impairment of the vascular wall these plaques develop.
This theory explains why human atherosclerosis
develops mainly at sites of altered hemodynamic conditions such
as the branching regions of coronary, cervical and cerebral arteries.
It explains why the primary manifestations of human CVD is myocardial
infarction and stroke, and also the increased risk of CVD associated
with hypertension, where an increased systemic pressure extensively
unmasks the underlying impairment of the vascular wall.
Figure b.
It is unlikely that Lp(a) primarily exerts its
atherogenicity by binding to the plasminogen receptor on endothelial
cells (27). These receptors are present throughout the vascular
system so that such a pathomechanism would lead to increased incidence
of peripheral vascular diseases and venous thrombi, which are
not necessarily associated with elevated Lp(a) plasma levels
Figure c.
Peripheral Forms of Atherosclerosis
We are now able to account for another phenomenon associated
with human CVD: The principle difference in the pathomechanisms
leading on the one hand to atherosclerosis at predisposition sites
and on the other hand to peripheral vascular disease (PVD). Myocardial
infarction and stroke are by far the most frequent manifestations
of CVD. The localized development of atherosclerotic plaques in
these patients can only be explained if the instability of the
vascular wall is the main risk factor. Elevated concentrations
of plasma risk factors, e.g., cholesterol or LDL, can not explain
the phenomenon of localized manifestation of CVD. They may, however,
play an aggravating role in the development of CVD in the individual.
In the development of PVD, however, these plasma
risk factors play a much more prominent role, exerting a direct
or indirect noxious effect on the vascular wall. Consequently,
this leads to atherosclerosis in the vascular periphery where
the contact between noxious plasma constituents and the endothelium
is prolonged. Triglyceride-rich lipoproteins, because of their
enhanced susceptibility to peroxidation, are such potential challengers,
leading to vascular damage in the periphery.
This theory explains the peripheral form of CVD
associated with Type-III hyperlipidemia, a metabolic disorder
in which triglyceride-rich lipoproteins accumulate in the plasma
as very low-density lipoproteins (VLDL) and intermediate-density
lipoproteins (IDL). These conditions are also characterized by
a further pathomechanism of lipid deposition in the vascular wall.
In addition to the extracellular deposition of Lp(a) described
above, the cellular uptake of oxidatively modified lipoproteins
by scavenger cells plays a more prominent role. This can also
explain why foam cells are found much more frequently in the vascular
wall of patients with these metabolic disorders.
A similar pathomechanism is involved in PVD associated
with cigarette smoking, Oxygen free radicals from the cigarette
smoke damage the endothelium directly or via oxidative modification
of lipoproteins. It is noteworthy that ascorbate, the strongest
antioxidant normally present in the human body, is also a potent
inhibitor of these pathomechanisms.
In general, inherited metabolic disorders resulting
in an elevated concentration of potentially noxious plasma constituents
are frequently associated with PVD, e.g., in homocystinuria.
Of particular interest is the pathogenesis of PVD
in diabetes mellitus. The glucose and ascorbate molecules share
structural similarities and compete for the same transport system
for cellular uptake. Elevated glucose levels competitively inhibit
an optimum tissue uptake of ascorbate, leading also to a chronic
ascorbate depletion of the vascular wall and its impairment. Therefore,
dietary supplementation of ascorbate should lead to an effective
control of diabetic angiopathy.
The different pathomechanisms leading on the one
hand to CVD at predisposition sites and on the other hand to PVD
are frequently interrelated. Nevertheless, their discrimination
described here may prove helpful for future therapeutic approaches.
Independent of the different pathomechanisms involved, ascorbate
deficiency is a common denominator of human CVD.
Prophylactic and Therapeutic
Considerations
The theory presented in this paper immediately suggests effective
prophylactic and therapeutic treatments for most individuals at
risk CVD and for CVD patients.
Prophylaxis.
Ascorbate, a potent reducing and hydroxylating agent has been
shown to be effective in achieving critical prophylactic aims:
lowering the plasma Lp(a) level, preventing Lp(a) deposition in
the vascular wall (16), decreasing elevated LDL levels (28), increasing
HDL levels (29), preventing oxidative modification of lipoproteins,
protecting against oxidative damage by scavenging oxygen free
radicals and by regenerating tocopherol, [ppteventing the oxidative
modification of lipoproteins (30), and, above all, preserving
the integrity of the vascular wall and preventing the formation
of atherosclerotic plaques (16).
Moreover ascorbate hits all these therapeutic targets
at the same time. It will be hard for any pharmaceutical product
to surpass ascorbate, a substance that has been developed and
improved by nature over billions of years. Premature atherosclerosis
is essentially unknown in most animals, whereas millions of humans,
with chronic ascorbate deficiency, die of atherosclerosis and
related diseases each year.
Therapeusis.
Ascorbate is able not only to prevent the formation of atherosclerotic
lesion but also to reduce existing plaques. It is well-established
that ascorbate increases HDL plasma levels, thereby promoting
reverse cholesterol transport by uptake of intra- and extracellular
lipid from the vascular wall.
On the basis of our finding that plaque development
is paralleled by the extracellular deposition of Lp(a) it is evident
that a major focus of therapeutic development is the release of
Lp(a) or its lipid component from the arterial wall. Ascorbate
may be involved in two ways: by dissociating apo(a) from the LDL-like
component of Lp(a), thus enhancing the lipoprotein efflux from
the vascular wall and by converting lysyl residues in this wall
into hydroxylysyl residues, thereby decreasing the binding affinity
to components of the vascular wall by way of the lysyl haptenic
group.
The efficiency of releasing Lp(a) from its bonds
to fibrinogen/fibrin in the vascular wall may be considerably
enhanced by administration also of small prophylactic doses of
one or more inhibitors that compete with the lysyl haptenic groups
[lysine, 6-aminohexanoic acid, p-aminomethylbenzoic acid, trans-4-aminomethylcyclohexane
carboxylic acid, and others].
For patients with advanced cardiovascular disease
therapeutic amounts of these inhibitors, together with ascorbate
and as adjuncts to appropriate conventional therapy, might be
prescribed, once their therapeutic effect has been clinically
proved.
It might be argued that this class of substances,
which are generally used as anti-fibrinolytic agents, might induce
coagulative complications. These substances are, however, protease
inhibitors and inhibit activation of fibrinolysis as well as the
activation of coagulation (31). These substances have been used
in long-term studies for different indications without compromising
side effects. We have, however, not found any earlier recommendation
of the use of these substances in the pharmacological treatment
of cardiovascular disease. The combination of these substances
with ascorbate may be considered ideal since ascorbate reduces
the need for further Lp(a) deposition in the vascular wall and
the inhibitors would enhance the release of already deposited
Lp(a). Moreover, ascorbate is known to have anti-coagulative (32)
and profibrinolytic properties.
Conclusion
The concept presented here offers for the first time a conclusive
explanation for the unique features of human CVD. It can answer
the questions that have remained yet unexplained by presently
available hypotheses on the development of CVD (1,2,3) Ascorbate
deficiency is a precondition as well as a common denominator of
CVD. With rare exceptions CVD is a degenerative disease. Its leading
risk factor is the instability of the vascular wall rather than
any plasma constituents, and its primary pathomechanism is the
deposition of Lp(a) and fibrinogen/fibrin in the vascular wall.
We can now explain why the strongest downward trend
in CVD mortality of all industrialized countries occurred in the
USA, the country with the highest vitamin C consumption. Moreover,
we now understand why these two developments exactly parallel
each other. On the basis of the scientific concept presented in
this publication it is now possible to achieve a similar success
also in other countries.
The pathomechanisms described here and the therapeutic
conclusions presented are the solution to the puzzle of human
cardiovascular disease.
We have discussed the following
points in detail:
the cause of today's most important disease by ascorbate deficiency,
the result of a genetic defect in combination with inadequate
intake of supplementary ascorbate;
the regulation of plasma Lp(a) levels by ascorbate and the reasons
why Lp(a) and ascorbate are found alternatively in most animal
species;
the identification of ascorbate deficiency as a common denominator
of endogenous and exogenous risk factors for CVD;
the conditions under which a physiological defense mechanism designed
by nature to limit the deleterious effects of ascorbate deficiency
can turn into a pathological process;
the extracellular deposition of Lp(a) and fibrinogen/fibrin as
the primary mechanism of human atherogenesis;
the details of a comprehensive theory of human cardiovascular
disease; and the difference between atherosclerosis at predisposition
sites and peripheral vascular disease;
finally, we presented prophylactic and therapeutic recommendations
made on the basis of these discoveries, which may lead to a breakthrough
for the prevention and treatment of human CVD.
50 years ago ascorbate deficiency was established as a prominent
risk factor in CVD (33), and 37 years ago ascorbate was shown
in preliminary angiographic studies to reduce atherosclerotic
plaques in man (34). There is no rational explanation why these
early observations of the therapeutic value of ascorbate were
ignored and did not become common knowledge in the medical profession
long ago.
Our publications have initiated further clinical
trials. The evidence of the beneficial effects of ascorbate available
now is already convincing but comprehensive clinical confirmation
should soon end the decades of reluctance and skepticism. We are
convinced that before long ascorbate will become the treatment
of first choice for cardiovascular disease.
The therapeutic significance of our discovery is
not limited to CVD; Lp(a) and ascorbate are involved in cancer,
inflammatory disease, and other diseases, including the process
of aging. The deposition of Lp(a) in the vicinity of disease can
be conceived as a defense mechanism to contain the progression
of disease, particularly at low ascorbate concentrations. The
Lp(a)-ascorbate connection is a regulatory principle of nature
that directly affects human health. Abolition of ascorbate deficiency
may profoundly improve human health and increase life expectancy
of human beings.
References
Rath M & Pauling L (1990): Proceedings of the National Academy
of Sciences USA 87, 6204-6207.
Brown MS & Goldstein JL (1984): Scientific
American 251, 58-66.
Ross R (1986): New England Journal of Medicine
314, 488-500.
Steinberg D, Parthasarathy S, Carew TE, Khoo JC,
& Witztum JL (1989): New England Journal of Medicine 320,
915-924.
Berg K (1963): Acta Pathologica 59, 369-382.
McLean JW, Tomlinson JE, Kuang WJ, Eaton DL, Chen
EY, Fless GM, Scanu AM & Lawn RM (1987): Nature 300, 132-137.
Brown MS & Goldstein JL (1987): Nature (London)
330, 113-114.
Rath M, Niendorf A, Reblin T, Dietel M, Krebber
HJ & Beisiegel U (1989): Arteriosclerosis 9, 579-592.
Niendorf A, Rath M, Wolf K, Peters S, Arps H, Beisiegel
U & Dietel M (1990): Virchows Archiv. A. Pathol. Anat. 417,
105-111.
Beisiegel U, Niendorf A, Wolf K, Reblin T &
Rath M (1990): European Heart Journal 11, Suppl. E., 174-183.
Seed BM, Hoppichler F, Reaveley D, McCarhty S,
Thompson GR, Boerwinkle E & Utermann G (1990): New England
Journal of Medicine 322, 1494-1499.
Dahlen GH, Guyton JR, Attar M, Farmer JA, Kautz
JA & Gotto AM Jr. (1986): Circulation 74, 758-765.
Zenker G, Koltringer P, Bone G, Kiederkorn K, Pfeiffer
K & Jurgens G (1986): Stroke 17, 942-945.
Hoff HF & Gaubatz JW (1982): Atherosclerosis
42: 273-297.
Gavish D & Breslow JL (1991): Lancet 337, 203-204.
Rath M & Pauling L (1990): Proceedings of the
National Academy of Sciences USA 87, 9388-9390.
Carlson LA, Hamsten A & Asplund A (1989): Journal
of Internal Medicine 226, 271-276.
Pauling L (1968): Science 160, 265-271.
Aulinskas TH, Van der Westerhuyzen DR & Coetzee
GA (1983): Atherosclerosis 47, 159-171.
Harwood HJ Jr, Greene YJ & Stacpoole PW (1986):
Journal of Biological Chemistry 261, 7127-7135.
Frei B, England L & Ames BN (1989): Proceedings
of the National Academy of Sciences USA 86, 6377-6381.
Ginter E (1973): Science 179, 702-704.
Beetens J, Coene M-C, Verheyen A, Zonnekyn L &
Herman AG (1986): Prostaglandins 32, 335-352.
Loscalzo J, Weinfeld M, Fless GM & Scanu AM
(1990): Arteriosclerosis 10, 240-245.
Harpel PC, Gordon BR & Parker TS (1989): Proceedings
of the National Academy of Sciences USA 86, 3847-3851.
Smith EB & Cochran S (1990): Atherosclerosis
84, 173-181.
Miles LA, Fless GM, Levin EG, Scanu AM & Plow
EF (1989): Nature 339, 301-303.
Ginter E (1979): Wld. Rev. Nutr. Diet. 33, 104-141.
Bates CJ, Mandal AR, Cole TJ (1977): Lancet 3,
611.
Jialal I, Vega GL & Grundy SM (1990): Atherosclerosis
82, 185-191.
Aoki N, Naito K & Yoshida N (1978): Blood 1,
1-12.
Bordia A & Verma SD (1985): Clinical Cardiology
8, 552-554.
Paterson JC (1941): Canadian Medical Association
Journal 44, 114-120.
Willis GC, Light AW & Gow WQS (1954): Canadian
Medical Association Journal 71, 562-568. |
