History of Polio Vaccine - and its Contamination with Monkey Viruses - including SCMV
by Professor John Martin - 1996
http://www.ccid.org/stealth/presentations/handout.html
Presentation at the"Twentieth Century Plagues" Symposium
Embassy Suites Hotel, Los Angeles International Airport, March 1, 1996
Marriott Hotel,San Francisco Airport, March 2, 1996.
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Overview: Stealth viruses are defined as cytopathic viruses able to establish a persistent infection because of deletion and/or mutation of specific genes which, if expressed, would evoke effective anti-viral cellular immunity (1-5). This presentation will mainly focus on stealth viruses derived from African green monkey simian cytomegalovirus (SCMV). Federal health authorities have been slow in addressing the potential transmission of stealth viruses in live polio viral vaccines.
Brief History of Poliomyelitis:
Epidemic paralytic polio began to appear towards the end of the 19th century
(6). The first report of a major outbreak was made by the Swedish pediatrician
Dr. Carl Medin in 1889. Polio epidemics soon appeared throughout Europe. Attempts
at animal transmission failed until 1908 when Dr. Carl Landsteiner (of blood
group fame), inoculated two monkeys with a spinal cord extract obtained at autopsy
from a 12 year-old boy. One monkey died acutely while a Rhesus monkey became
paralyzed.
A major outbreak of paralytic polio occurred in the United States in 1916 affecting
nine thousand individuals in New York City (7). Each summer there were reported
clusters of polio in various parts of the United States. An unusual polio-like
illness affected California in 1934. One hundred and ninety eight medical personnel
at the Los Angeles County Hospital became sick (6). They were not paralyzed,
but instead developed a chronic fatigue syndrome (CFS)-like illn176" Attempts
to isolate polio virus were unsuccessful. A class action suit was settled in
1938 for several million dollars, supposedly with the stipulation that there
be no publicity to suggest that caring for polio patients could possibly be
hazardous.
Basic studies showed that (i) polio virus initially infected the alimentary
tract; (ii) Only a small percentage (<1%) of infected individuals actually
developed paralysis; (iii) there were 3 serologically distinct Types (1, 2 and
3); (iii) most cases of paralytic polio were due to Type I, as exemplified by
the highly virulent Mahoney strain; (iv) serum from a previously infected individual
contained protective type-specific antibodies; (v) polio virus could be passed
in monkey and mouse brains but "brain adapted" polio did not grow
well in non-nervous tissues (6).
A major breakthrough occurred in 1948 when Dr. John Enders showed that by using
antibiotics, it was possible to culture intestinal cells on which polio virus
could be propagated and could produce a quantifiable cytopathic effect (CPE).
Development of Polio Vaccines: There were two competing approaches to vaccine
development. The influenza vaccine model involved the use of inactivated (killed)
virus. The yellow fever vaccine model involved the use of a weakened or attenuated
strain as a live viral vaccine. Several unsuccessful efforts were made in the
1930's using these approaches with the polio virus grown in monkey or mouse
brain.(6).
Following the work of Dr. Enders, Dr. Jonas Salk was commissioned in 1953 by
Basil O'Connor, Director of the National Foundation for Infantile Paralysis
(March of Dimes Foundation), to produce an inactivated polio vaccine (IPV).
Dr. Salk grew virulent polio viruses on Rhesus monkey kidney cells and inactivated
the harvested viruses using a 1:4,000 dilution of formaldehyde. Serious questions
concerning (i) the necessity of using the Mahoney isolate for Type 1 polio,
(ii) the dynamics and completeness of formaldehyde inactivation and (iii) statistical
analyses of the early trial data using experimental vaccine lots were smothered
by O'Connor's powerful Public Relations campaign and by the public's eagerness
for a vaccine. The Federal Laboratory of Biological Safety (a component of the
National Institutes of Health) licensed polio vaccine on April 12, 1954. This
occurred in spite of Dr. Bernice Eddy notifying her supervisors that several
monkeys developed paralysis from the vaccine made at Cutter Laboratories.
Soon after the launching of the commercial vaccine lots in April 1955, there
were 10 deaths and 192 cases of vaccine induced paralytic polio. Most of the
cases were traced to the Cutter vaccine. Vaccine lots from Park Davis and Eli
Lilly were also found to contain live virus and the Industry knew that Dr. Salk's
assumptions about formaldehyde were invalid. Efforts were made to single out
Cutter as the only defective vaccine, while at the same time improve upon the
inactivation protocol. The vaccine program was halted on April 27th and resumed
on May 27th, hopefully still in time for the anticipated July onset of natural
polio cases. By November, new manufacturing safeguards were introduced, such
as an additional filtering step, without any recalls of existing lots. The Laboratory
of Biological Safety was reorganized and placed under the Food and Drug Administration
(FDA) as the Division of Biological Standards. For her good work, Dr. Eddy was
removed from polio vaccine testing!
Although the efficacy of IPV was exaggerated by changing the clinical definition
of paralytic polio and other maneuvers, it led to a significant reduction in
polio cases. It still probably caused several cases from residual live virus.
Public Health critics of the program were shunned and their protests nullified
by legislating compulsory vaccination. Dr. Albert Sabin, Dr. Hilary Koprowski
and others were more interested in developing an attenuated polio virus which
could be administered as a live vaccine. Dr. Koprowski conducted extensive human
and animal trials in Central Africa. A 1956 trial in Ireland was marred by the
occurrence of polio in vaccine recipients. Dr. Sabin had more success, mainly
because he made use of Dr. Renato Dulbecco's technique of plaque purifying attenuated
viral isolates. By 1960, Dr. Sabin had convinced much of Europe that his vaccine
was less expensive and created more rapid and longer lasting immunity than did
IPV. Moreover, excretion of live vaccine virus indirectly vaccinated others
within a community and helped out-compete virulent viral strains.
The subtle nucleotide changes, mainly within the 5' non-coding region, that
distinguish attenuated from wild type virus have recently been identified. Much
of the difference involves a single nucleotide substitution. The attenuated
strains can revert to more pathogenic variants, and even approved vaccine lots
contain some revertants. This problem occurs more frequently with the least
altered, Type 3 polio vaccine strain.
SV40 Contamination: From 1957 Dr. Eddy was involved in pioneering work with
Dr. Sarah Stewart on the ability of a mouse Polyoma virus to induce tumors in
hamsters. Dr. Eddy was suspicious that monkey kidney cells might have a polyoma-like
virus. In April 1960, she reported to her supervisor, Dr. Joseph Smadel, that
extracts from Rhesus monkey kidneys induced tumors in hamsters similar to those
induced with Polyoma virus. Her work was dismissed by Dr. Smadel. Moreover,
she was severely chastised for subsequently mentioning her findings at a Polyoma
virus conference held in New York in August, 1960. She was instructed that all
future utterances had to be written and submitted for approval by Dr. Smadel.
Dr. Maurice Hillerman of Merck was also concerned that the Rhesus monkeys being
used for polio vaccine were becoming increasingly infected with unknown viral
agents. He asked the Director of the Washington D.C. Zoo to arrange a shipment
of a different species of monkey, imported separately from the usual routing.
He received African green monkeys from Africa via Madrid and Baltimore. Extracts
from Rhesus monkeys produced a strong vacuolating cytopathic effect on the African
green monkey kidney cells. The responsible virus was the 40th virus isolated
from Rhesus monkeys and called SV40. It was subsequently shown to be the same
virus as found by Dr. Eddy to cause cancer in hamsters.
SV40 is endemic in Rhesus monkeys, producing very little CPE. It does not occur
naturally in African green monkeys and when present, it produces a strong CPE.
With suppressed publicity, FDA undertook a major effort to switch the polio
vaccine seed lots from Rhesus to African green monkeys using anti-SV40 antibodies
to neutralize the contaminating virus. Brief and belated mention of the problem
occurred in the press; even Dr. Eddy was subsequently allowed to publish her
findings. She had, however, lost her laboratory and her research support.
The SV40 issue was initially seen as a problem for the live viral vaccine. Unfortunately,
the virus was not inactivated by 1:4,000 formaldehyde and parental inoculation
created more infections than oral administration. However, since there were
no apparent ill effects, the concern over this virus subsequently waned. Yet,
recently there have been reports of SV40 virus in both childhood choroid plexus
brain tumors (8) and in mesotheliomas (9). The children were too young to have
received SV40 directly from a vaccine and in all likelihood this virus is now
circulating within the human population.
Live polio virus vaccine was licensed to Lederle (American Cyanimid) as Orimune(R)
in 1961 and has since largely replaced inactivated vaccines. Occasionally (8-10
cases per year in the United States), the Type 3 vaccine polio reverts to virulence
and induces disease. \
Viral Contamination of Live Polio Virus Vaccines: During early vaccine
developments almost 50% of the kidney cultures established for polio vaccine
production were discarded because of obvious viral contaminants (mainly foamy
retroviruses but also adenoviruses and non-identifiable agents). Few if any
of these adventitious agents were thought to be pathogenic for man. An exception
was the monkey B virus, a herpes simplex-like virus known to cause a fatal encephalitis.
Another major scare arose in 1968 in Marburg, Germany when monkeys intended
for vaccine production transmitted an acute hemorrhagic illness to their caretakers.
Renewed efforts went into screening for unknown viruses. In 1968, Dr. Kendall
Smith, an electron microscopist at FDA Division of Biological Standards, detected
viral-like agents in some batches of polio vaccines. He unsuccessfully argued
for the use of a fluorescence focus assay using sera from monkeys tested on
their own kidney cell cultures. Consideration was given by Lederle to switching
from monkeys to human cells for vaccine production. This approach was taken
by Pfizer, an English pharmaceutical company. Their product was called Diplovax
and was derived from human diploid cells.
In a joint Lederle/Bureau of Biologics study conducted in 1972 "All eleven
monkeys studied demonstrated the presence of CMV-like agents. These monkeys
all originated from Kenya over a short period of time. Seven of these monkeys
would have passed our existing test standards." In a "Cytomegalovirus
Contingency Plan", dated August 4th, 1972, Dr. Vallancourt from Lederle
argued that "Unless and until Pfizer's Diplovax is in abundant supply,
the BB [Bureau of Biologics] cannot risk Lederle being off the market."
On March 16th, 1973, Dr. Vallancourt wrote to the President of American Cyanamid,
"I do not believe our problems with the slow release of specific lots of
Orimune(R) are a result of a Pfizar influence..... Furthermore, if the Bureau
wanted to restrict us they could bring up the subject of CMV (Cytomegalovirus)
in our substrate (i.e. African green monkey kidney tissue) which they have not
done, even though they have told us the monkeys in the collaborative study performed
in 1972 were all positive for this agent."
In 1977 assays for retroviral reverse transcriptase activity were applied to
some polio vaccines. Certain vaccine lots tested positive and this activity
could be transmitted to cell cultures which developed an atypical CPE. It is
now known that many of the African green monkeys used were infected with simian
immunodeficiency virus (SIV). Interestingly, African green monkeys brought to
the Caribbean earlier this century were not infected with SIV, raising the possibility
that SIV is a more recent infection than generally thought and possibly of experimental
vaccine origin. Discussion at the time of possible Type C retroviruses in polio
vaccines led to more detailed electron microscopy. Particles were seen in polio
batch 3-444, but were considered more likely to be cell debri than actual viruses.
I worked at the time as Director of the Viral Oncology Laboratory at the Bureau
of Biologics. In 1978, Dr. G. Aulakh and I confirmed that a bulk monopool of
polio vaccine contained a considerable amount of DNA, not all of which could
be accounted for as simple cellular debri. I was not provided any information
on the earlier concern about CMV, but was told that the monopools were submitted
only to determine if they met the mutually approved and mandated tests for polio
vaccines. In other words, they were not available to continue this line of experiments.
I still remember the project terminating statement from the Bureau's Director:
"Stop worrying about it, every time you eat an apple you ingest foreign
DNA."
The issue of probable contamination of polio vaccines with adventitious viruses
was difficult for anyone to contradict. Maintaining support for the established
vaccine program was, however, variously argued: (i) The continued use of primary
cultures from kidney cells would help avoid any suggestions that established
cell lines may have progressed towards cancer and may contain "oncogenes".
(ii) The polio vaccine had been administered to many millions of individuals
without apparent adverse effects. It was, therefore, unnecessary and anyhow
too late, to correct the situation; (iii) The viruses detected were not the
dreaded Marburg agent or the much feared Type C cancer associated retroviruses
and were, therefore, of little significance and were probably destroyed when
passing through the stomach; (iv) The pharmaceutical industry had to be encouraged
to manufacture vaccines and the public had to be encouraged to take vaccines
for the government-sponsored immunization programs to be successful. (v) The
programs were predicated on existing costs and profit margins and could be threatened
if additional testing was imposed. (vi) Many companies had ceased vaccine manufacturing
within the United States and any further reduction could make the country more
vulnerable to threatened germ warfare, etc., etc.
Neuropsychiatric Illnesses: It is generally believed that the incidence of chronic
brain dysfunctional disorders has steadily increased over the last several decades.
Conditions such as chronic fatigue syndromes, fibromyalgia, migraine, attention
deficit hyperactivity disorder, autism, mental depression, dementia, schizophrenia,
etc., are being increasingly diagnosed. Our society has somewhat complacently
accepted these conditions as inevitable consequence of "progress".
Moreover, compared to efforts aimed at clinical management of these diseases,
relatively little effort has gone into identifying their etiology. The involvement
of basic researchers has been especially hampered by the imposition of confusing
clinical case definitions. Medical specialists have somewhat arbitrarily segregated
various facets of neuropsychiatric illnesses into a wide array of nosologically
distinct, territorily protected, clinical entities. The ever increasing multiplicity
of named dysfunctional brain syndromes may simply reflect the complexity of
the brain, rather than imply the presence of innumerable etiologic processes.
Search for Viral Infections in Neuropsychiatric Diseases: I initiated
a project in 1986 to see if patients diagnosed as having the chronic fatigue
syndrome (CFS) were virally infected (1). Early findings using the polymerase
chain reaction (PCR) with primer sets cross-reactive with all of the known human
herpesviruses gave weak positive signals with one third of CFS patients, but
not with any of several laboratory controls (10). I later found that many CFS
patients would also give low, but detectable PCR responses using primers designed
to amplify the tax gene of human T lymphocytotropic viruses.
The potential significance of the marginal responses seen in CFS patients became
clearer in 1990 when strikingly positive PCR responses occurred with cerebrospinal
fluid (CSF) samples from two patients and on a brain biopsy of a third patient.
All three patients had unexplained severe encephalitis-like illnesses. The brain
biopsy came from a school teacher who had gradually lost her capacity for written
and oral communication, but was otherwise alert with no localizing neurological
signs. She did, however, have an abnormal MRI with periventricular lesions.
The brain biopsy showed mild gliosis with no inflammation. Complete and incomplete
forms of herpesvirus-like particles were present in several of the glial cells.
Some of the virus positive cells showed marked vacuolated changes and lipid
accumulation (11). The PCR positive CSF samples were acellular, indicating an
absence of inflammation. One had come from a newborn infant with delayed neural
development. The other from an adolescent with residual severe brain dysfunction
following what was called an atypical herpes simplex encephalitis.
From about 1987, I had devised several approaches to try to grow human herpes
virus-6 (HHV-6) from CFS patients using cord blood lymphocytes. Routine human
fibroblast cultures were also established. The latter cells frequently showed
a delayed, transient CPE somewhat suggestive of human CMV. Buoyed by the PCR
findings in the severe encephalopathy cases, efforts were again undertaken to
culture a virus from a PCR positive CFS patient (D.W.). After 6 weeks of culture,
enlarged, rounded, vacuolated cells suddenly began to appear in both human and
monkey derived cell lines. Cell syncytia were easily recognized. The CPE could
be passed to many other cell types and to cells of multiple species. By electron
microscopy, numerous complete and incomplete herpesvirus-like viral particles
were seen. The foamy, vaccuolated cells did not, however, stain with antisera
specific for the immediate-early gene of human CMV. Nor did the cells stain
with antisera specific for HSV, HHV-6/7, VZV or adenoviruses. PCR assay using
the HTLV tax gene primer gave two well defined products. Sequencing of one of
the PCR products (GenBank accession # U09212) identified a region of partial
sequence homology to the UL34 gene of human CMV. The sequence of the other PCR
product (GenBank accession # U09213) was suggestive of a possible herpesvirus
origin but could not be aligned with any of the known herpesviruses (3). Viral
DNA was isolated and cloned. A region of sequence homology to African green
monkey simian cytomegalovirus (SCMV) was first found in early 1994. Unrelated
to our work, Dr. Gary Hayward of Johns Hopkins University submitted additional
sequence data on SCMV to GenBank in December 1994. From his sequence data, it
was unequivocal that the CFS patient's virus had originated from SCMV (5).
In 1991 I coined the term "stealth" to describe the viruses I had
been seeking. I used this term primarily because it carried the connotation
that the viruses could occur in the absence of inflammation. The SCMV-derived
virus was designated stealth virus-1. A closely related virus (stealth virus-2)
was isolated in early 1991 from the CSF of a patient with an acute severe encephalopathy
following a 4 year history of a manic depressive illness. The patient (B.H.)
has remained in a vegetative state since 1991. DNA sequencing of a PCR amplified
product from her infected cultures has identified the virus as being similar
but not identical to the SCMV-derived stealth virus-1. Numerous other stealth
viral isolates have been obtained and are awaiting resources to perform the
necessary sequencing analyses.
Animal Studies: Stealth virus-1 induces an acute neurological illness when inoculated
into cats (12). The early manifestations developed within a week and included
gingivitis, bloody ocular and nasal discharge, lymphadenopathy, pupil dilatation
with photophobia (squinting in response to light) and nuchal hair loss from
rubbing against the cage. There was a reduction in body temperature beginning
in the second week which averaged 0.6oF at 2 weeks and 0.8oF at weeks 3 and
4. Most striking was the marked behavioral changes in all of the virus-inoculated
cats. They lost the playfulness that was present prior to injection and became
reclusive and irritable. They resisted being handled and the animal caretakers
resorted to wearing leather gloves. By palpation, the enlarged lymph nodes and
various muscle groups were identified as being painful for the animals. The
severity of the illness peaked at around 4 weeks with definite improvement noted
in the cat necropsied at 6 weeks. A cat that was maintained to 15 weeks had
resumed normal activities by week 10 and appeared to be symptom free. Histological
examination of animals' brain tissue showed foci of cells with cytoplasmic vacuolization
and an absence of any inflammatory reaction. Electron microscopy on several
cats confirmed the presence of occasional herpes-like viral particles and, more
commonly, the presence of variable patterns of accumulations of viral-like granular
and other membranous structures suggestive of subgenomic viral expression.
Unstable, Fragmented Nature of the Stealth Virus-1 Genome: Restriction enzyme
digests of stealth virus-1 have been cloned and partially sequenced. The genome
appears to comprise multiple fragments of approximately 20 kilobase pairs. The
virus displays an unusually high degree of sequence microheterogeneity suggesting
infidelity of DNA replication or an alternative replication strategy (13). The
concept of a fragmented, unstable viral genome is consistent with electron microscopic
observations (14). It has important implications for the approaches to be taken
in using molecular techniques to screen for these viruses. It also raises concerns
about the possible oncogenicity of stealth viruses (16).
Stealth Viruses Isolated from Patients with Severe Encephalopathy: Since the
beginning of these studies, a number of patients have been identified with strongly
positive cultures and complex clinical case histories. While the initial focus
was on CFS patients, the more recent emphasis has been on patients with severe
encephalopathy. In many of these cases, a preceding CFS-like illness was present.
The clinical observations support the concept of potentially infectious neuropsychiatric
illnesses attributed to varying degrees of dysfunction of different regions
of the brain (2). Brain biopsies have been obtained in five patients and have
shown many of the characteristic changes noted in the infected cats. In some
of the biopsies, there is an additional vasculitis component. Possibly, the
most promising clinical aspect of these illnesses is the recovery process seen
in several, but not all, severely ill patients. The mechanism of recovery is
the most important goal of stealth virus research. In a step towards this goal,
I am hoping to obtain sufficient sequence data on isolates from severely ill
adult patients and from autistic children, to determine which, if any, have
originated from African green monkeys. I realize that while monkey cells have
been used for polio and adenovirus vaccines; dog and duck kidney cells have
been used for rubella vaccines; chicken cells have been used for measles and
mumps vaccines; and a very wide range of animals cells have been used for animal
vaccines. Unfortunately, only limited sequence data are available on most animal
viruses. Some stealth viruses may simply have originated by the down sizing
of known human viruses, especially human herpesviruses. In these endeavors,
I have so far unsuccessfully sought the help of both the FDA and the CDC.
Notification to CDC, FDA and Lederle: CDC was notified in early 1991 that a
repeat positive culture was obtained on patient D.W. and a similarly positive
culture was obtained on the comatose patient B.H. An invitation to visit my
laboratory to see the cultures was declined. CDC was again notified in mid 1994
when the sequence data on stealth virus-1 showed a greater relatedness to SCMV
than human CMV. FDA Center for Biologics Evaluation and Research (CBER) was
contacted in March of 1995 and the President of Lederle sent a letter in July,
1995. Prompted by FDA personnel, unsolicited requests for collaborative and
financial assistance were sent to CDC and to FDA in June 1995, followed by visits
to both agencies. The unsolicited proposal format is designed to protect an
agency from the accusation that it has given a competitive advantage to someone
seeking government funds. The proposals included detailed clinical descriptions
of 12 cases of severe, otherwise unexplained, encephalopathy. In the FDA proposal,
I asked to do a surveillance study to determine the prevalence of simian CMV-derived
stealth viruses in humans and in the monkeys used for polio vaccine production.
I also wanted to test some vaccine monopools. In the CDC proposal, I asked for
help in sequencing the viral isolates from the 12 patients.
Response from CDC Received 5 Months After Submission: "Reviewed by the
National Immunization Program (NIP) and the National Center for Infectious Diseases
(NCID) of CDC. It was determined that the proposal did not address NIP research
needs at this time. There was also the comment from NCID that "The twelve
patients reported have variable clinical histories with no obvious epidemiological
links between them. The evidence that a virus can be isolated from these cases
is unconvincing. No independent confirmation has been reported in the results
described in this proposal and the evidence for the existence of an infectious
agent which the offeror (sic) calls a 'stealth virus' remains unconvincing."
Unofficially, I was told that Ms. Joanne Patton, now working in Dr. John Stewart's
laboratory at NCID, recalled hearing of a patient becoming infected with SCMV
which had contaminated a rubella virus vaccine grown on African green monkey
cells. From discussions with Ms. Patton and Dr. Stewart, there seems to be some
regret that CDC had not made efforts to pursue this event. A request for a brief
statement in the Mortality and Morbidity Weekly (MMWR) on atypical viral encephalopathy
was also denied.
Response from FDA Received 7 Months after Submission: "Request for support
to screen for the prevalence of simian cytomegalovirus derived stealth viruses
in humans is best sought from an agency such as the NIH, rather than the FDA.Requests
to screen the monkey colonies that are used in vaccine production for the presence
of stealth viruses. These are studies that would need to be conducted with the
manufacturers.
Request to screen polio samples (the bulk mono-pools) for stealth viruses. Screening
of these samples, if done, should be carried out in CBER's own laboratories.
We are evaluating the types of studies that might be best done using PCR-based
techniques. However, even if such sequences are found in a PCR-based assay,
the question whether transmissible, replication competent viruses are present
would still need to be addressed.
We appreciate your informing us and others, not only in your submitted proposal
but also at the FDA Workshop on cell substrates and at the IOM meeting on vaccine
safety, about your concerns vis-a-vis simian cytomegalovirus and potential related
viruses in the polio vaccine. We will be addressing this concern in our Laboratories".
Other Relevant Actions: The Advisory Committee on Immunization Practices (ACIP)
had made a recommendation to move from a series of four injections of live polio
vaccine to a split protocol of two injections of inactivated vaccine (IPOLTM,
produced by Pasteur Merieux-Connaught Laboratories) followed by two injections
of live vaccine. This was obstensibly to help reduce the occurrence of the approximately
8-10 cases a year of poliomyelitis from Type 3 vaccine revertants. Although
not cited as a reason, such a move would expand the production of inactivated
vaccines should a subsequent total switch to inactivated vaccine be recommended.
A decision to delay the implementation of this plan was made at the February
ACIP meeting. There will be opportunity for public input at the June meeting.
FDA has held open meetings to discuss possible hazards of interspecies bone
marrow therapy in AIDS patients and interspecies liver and other organ transplants.
FDA was unable to muster support to restrict the first baboon bone marrow trial.
Summary: The concepts that certain stealth viruses may have arisen as contaminants
of live viral vaccines, and that vaccinations may have had untoward consequences,
have not been embraced by either vaccine manufacturers or Public Health agencies.
As the experimental data unfold, however, the existence and the clinical importance
of stealth viral infections are less easily reputed. Indeed, stealth viral infections
may explain a wide range of neurological and neuropsychiatric diseases, serving
as a common thread linking these diseases, and possibly accounting for their
ever increasing prevalence.
If a vaccine program were to be initiated today, one would surely not import
wild monkeys from Africa, create short term primary kidney cultures, add a human
virus and administer the crude gamish derived from the virally infected cells
to virtually every child in the country. Nor would one want to withhold applying
the many molecular biological techniques developed over the last 30 years to
assess vaccine purity. Yet this is essentially the situation with live polio
vaccine and comparable arguments can be made for other human and animal viral
vaccines.
Various meetings, phone calls and document exchange have uncovered a sense of
frustration within the Federal Public Health System, Industry, and the general
public with what appears to be a resistance of those in authority to face the
issue of prior, if not also present, vaccine contamination. If animal viruses
have been inadvertently introduced into humans, the sooner we find out the better.
I would very much appreciate continuing to hear about patients with seemingly
complex infectious and/or neuropsychiatric illnesses. Volunteers are needed
to help bring these patients to the attention of the Public Health System. Work
on the in vitro efficacy of stealth virus inhibitors needs support so that clinical
therapeutic trials may soon become a reality. Phone and FAX messages can be
left at 818 799-4500 and 818 799-1700 in the Los Angeles area and at 510 222-9466
and 510 222-9466 in the San Francisco area. The e-mail address is wjmartin@mizar.usc.edu
References
1. Martin W.J. Viral infection in CFS patients.
in "The Clinical and Scientific Basis of Myalgic Encephalomyelitis Chronic
FatigueSyndrome." Byron M. Hyde Editor. Nightingdale Research Foundation
Press. Ottawa Canada pp 325-327, 1992.
2. Martin W.J. Stealth viruses as neuropathogens.
CAP Today 8 67-70, 1994.
3. Martin WJ, Zeng LC, Ahmed K, Roy M. Cytomegalovirus-related
sequences in an atypical cytopathic virus repeatedly isolated from a patient
with the chronic fatigue syndrome. Am J Path. 145: 441-452, 1994.
4. Martin WJ. Stealth virus isolated from an autistic
child. J Aut Dev Dis. 25:223-224, 1995.
5. Martin WJ, Ahmed KN, Zeng LC, Olsen J-C, Seward
JG, Seehrai JS. African green monkey origin of the atypical cytopathic 'stealth
virus' isolated from a patient with chronic fatigue syndrome. Clin Diag Virol.
4: 93-103, 1995.
6. Paul JR. A history of poliomyelitis. Yale University
Press, New Haven, 1971.
7. Gould T. A summer plague. Polio and its survivors.
Yale University Press. New Haven, 1995.
8. Lednicky JA et al. Natural simian virus strains
are present in human choroid plexus and ependymoma tumors. Virology 212: 710-717,
1995.
9. Cristaudo A, et al. Molecular biology studies
on mesothelioma tumor samples: preliminary data on H-ras, p21 and SV40. J. Environ
Path 14: 29-34, 1995.
10. Martin WJ: Detection of viral related sequences in CFS patients using
the polymerase chain reaction. In Hyde B ed. The Clinical and Scientific Basis
of Myalgic Encephalomyelitis/Chronic Fatigue Syndrome. Nightingale Res Found.
Ottawa Canada, pp278-282, 1992.
11. Martin WJ. Severe stealth virus encephalopathy following chronic fatigue
syndrome-like illness: Clinical and histopathological features (submitted)
12. Martin WJ, Glass RT. Acute encephalopathy induced in cats with a stealth
virus isolated from a patient with chronic fatigue syndrome. Pathobiology 63:
115-118, 1995.
13. Gollard RP, Mayr A, Rice DA, Martin WJ. Herpesvirus-related sequences
in salivary gland tumors. J Exp Clin Can Res.15: 1-4, 1996.
14. Martin WJ. Genetic instability and fragmentation of a stealth viral
genome. Pathobiology (in press).
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