What Causes a Positive Test for HIV-Antibodies?

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  • Vladimir Koliadin

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  • -

Category

  • HIV Tests

Topic

  • HIV Test Accuracy

Article Type

  • Editorial Article

Publish Year

  • 1999

Meta Description

  • Studies show HIV tests' high specificity but don't prove HIV's existence. False positives are rare. Some argue tests' use as diagnostic tools needs review.

Summary

  • The content discusses the issue of HIV-positivity and its relationship to AIDS. It questions the validity of studies that claim HIV-positivity is specific to AIDS, pointing out that the control group in these studies was not properly matched to the AIDS group. The importance of matched control groups in scientific studies is emphasized. The content also highlights the presence of non-specific immunoglobulins in the body and their potential to yield false positive HIV tests. It explains that only a portion of immunoglobulins produced in response to an antigen are specific, while the majority are non-specific. The problem of non-specific immunoglobulins is further exacerbated in certain HIV test systems. The content concludes by stating that the available evidence suggests that HIV antibody tests are not standardized or reproducible, and the proteins considered specific to HIV may actually be normal cellular proteins. It questions the specificity of the Western Blot test and suggests that a positive result may be due to cross-reactivity with non-HIV antibodies.

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  • HIV

  • AIDS

  • HIV-antibodies

  • HIV-seropositivity

  • HIV-tests

  • Specificity

  • Western Blot (WB) test

  • ELISA systems

  • False positive

  • Antigen

  • Immunoglobulins

  • T4-lymphocytopenia

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By Vladimir Koliadin
April 1998 (Revised June 1999)

Introduction

In 1993, the widely accepted ideas that a positive test for HIV-antibodies is specific (i.e. means HIV-infection) and that HIV exists as an exogenous retrovirus were challenged by Papadopulos-Eleopulos et al. (Perth Group) [1]. Then these views were developed by the same [2] and other authors [3,4]. Neither experimental nor even logical arguments were advanced by mainstream AIDS-scientists to disprove the central points of the Perth Group [1,2] *. At present, it is still accepted in mainstream AIDS-science that existence of HIV and high specificity of HIV-antibody tests are ultimately proven scientific facts. Besides conformity of thinking and vested interests, this belief is maintained due to the absence of clear-cut alternative explanations for the phenomena which are thought to prove the HIV-causes-AIDS theory. Some important questions have not been answered. If HIV does not exist, what causes a positive test for HIV-antibodies? Why are almost all AIDS-patients seropositive while almost all healthy individuals are not? Why is the positive test strongly associated with high mortality and susceptibility to opportunistic infections?

At the heart of any HIV-antibody test are the so called HIV-proteins. These proteins are produced by cell-cultures of human lymphocytes. According to the mainstream AIDS-science, these proteins belong to a new retrovirus HIV, by which these cell-lines are presumably infected. HIV-skeptics say that these proteins are of endogenous (intracellular) nature [1]. Following the facts and basic principles of immunochemistry, the only conclusion which may be drawn from a positive test for HIV-antibodies is that some immunoglobulins in the tested blood-serum have bound to these "HIV-proteins". This is the case for both ELISA and Western Blot (WB) tests, as well as for any other immunochemical test. The point of disagreement is how to interpret such binding. Mainstream science insists that such binding is due to specific antibodies, produced by the immune system after it comes in contact with HIV. The Perth Group [1,2] explain this binding by cross-reactions between "HIV-antigens" and antibodies to other non-HIV antigens, to which AIDS- patients and individuals from high-risk groups are exposed. Such cross-reactions are well known to occur when different antigens share common parts ("antigen determinants"). In this case, antibodies to one such antigen are capable of binding selectively to another antigen with the same antigenic determinants. Nevertheless, the cross-reactivity hypothesis suffers from one problem: how to explain that almost all AIDS-patients and many people in high-risk groups have been exposed to some antigens bearing common determinants only with "HIV-antigens"? Why almost everyone beyond the risk- groups have not been exposed to such antigens, although anyone in the course of his/her life has been exposed to many antigens (vaccinations, infections, etc.)?

1. Why HIV-antibody tests are thought to be specific

In the middle of the1980s, it was shown experimentally that a test for HIV-antibodies is positive in a great proportion of patients with a diagnosis of AIDS or pre-AIDS, while it is negative in almost all perfectly healthy individuals. It should be noted that AIDS-diagnosis in these patients was established from clinical symptoms, not from the HIV-test itself. This undermines the "circular definition" argument advanced by some AIDS-dissidents. Moreover, such studies were carried out according to a blind and randomized protocol [9]. This gave great credibility to the HIV-causes-AIDS viewpoint. Do such studies actually prove that HIV- positivity is specific to AIDS? Even though it may seem "self-evident" at first sight, it is not so. An important principle of evidence-based science was obviously violated in these studies: the control group was not matched to the AIDS group - perfectly healthy individuals were used as controls [1].

Why is the principle of matched control so important? The following simple example may help illustrate why. Take a disease that is characterized by some feature, say by elevated body temperature. A study shows each of 1,000 patients with this disease demonstrates high temperature, whilst each of 1,000 healthy controls - normal (lower) temperature. Does it mean that elevated body temperature is specific to this disease? Surely not - simply because the high temperature, though being highly unusual in healthy individuals, is typical to many other diseases. For the same reasons, the ability of HIV-test to discriminate between AIDS-patients and healthy individuals cannot prove specificity of HIV-tests. This obvious flaw in the studies of "specificity of HIV-antibody tests", spotted by the Perth Group [1], was ignored by the mainstream science. Which symptoms in AIDS-patients should be matched in the control group? It is not an easy question: many symptoms and signs are typical to AIDS. The Perth Group did not specify such symptoms. In the next section an attempt will be made to fill this gap.

Among other studies carried out with large number of individuals (applicants for US military service) specificity of HIV-tests has been reported as high as 1 false positive reaction in more than 135,000 [5]. Nevertheless, these studies have nothing to do with proofs of existence of HIV or specificity of HIV-antibody tests because only WB test systems were used as the "gold standard" of HIV. All these studies demonstrated is that results provided by some ELISA systems in multistep testing algorithms are well compatible with results of WB tests, at least in a population with a predicted very low prevalence of HIV-seropositivity. The unknown specificity of the "confirmatory" WB-tests themselves was not addressed in these studies.

2. Non-specific immunoglobulins as the cause of HIV-seropositivity

The B-lymphocytes (a part of the immune system) normally respond to foreign substances (named "antigens") by increased production of special proteins - immunoglobulins. Some of these immunoglobulins are capable of specific binding to the antigen - that is, they bind strongly to the antigen but not to other substances. Such immunoglobulins are usually named "antibodies". Other immunoglobulins, which are capable to bind to a wide range of antigens, are named "non-specific immunoglobulins". Many authors name all immunoglobulins "antibodies"; to discriminate between the two types they use the terms "specific antibodies" and "non-specific antibodies" (or "normal antibodies"). The ability of (specific) antibodies to bind only to the antigen which induced production of these antibodies plays a very important role in biomedical science and serological testing.

If HIV-antibody tests are positive in AIDS-patients and negative in healthy controls, does it mean that blood-serum of AIDS patients contains some factor which is absent in healthy individuals? Most scientists (aside from specialists in practical immunochemistry), let alone laymen, may believe that at least this fact was proven beyond any reasonable doubt by such studies. Nevertheless, this is not the case: blood-serum from healthy individuals is also capable of testing positive by WB. The only difference is that titers of this reaction are higher for AIDS-patients than for healthy controls. The titer is the maximal dilution of the serum for which reaction is still noticeable. For example, R.Gallo and his group managed to obtain "specificity" (in respect to healthy controls) only after 500-fold dilution of the serum [6,7]. Thus, blood serum from healthy controls provides positive WB-test results when diluted less than 1:500. In practical immunochemistry, such a phenomenon is explained by binding of non-specific immunoglobulins, which are present in any individual and bind to almost any antigen. In commercial WB-systems this effect is not noticeable because sensitivity is artificially lowered to avoid positive reactions in healthy individuals.

How to decide whether a test is positive because of binding with specific antibodies or only with non- specific immunoglobulins? In the practice of immunochemical testing this problem is apparently resolved by reduction of sensitivity (e.g. by dilution of the tested serum) up to the levels which guarantee negative tests in healthy controls. Such an approach tacitly implies that reactivity and concentrations of non-specific immunoglobulins are about the same in all individuals. Even though being widely accepted, this practice is dubious. If some states of organism are characterized by essentially higher levels of non-specific immunoglobulins or by their higher affinity (ability to bind), blood serum from such individuals can yield a positive test too. How to prove that a positive test for a given sample is caused just by specific antibodies, but not by non-specific immunoglobulins? By definition, specificity of antibodies means they are capable of binding only to one antigen (or very similar ones). Hence, it is necessary to check how this serum reacts with a great many of other antigens. If titers of these reactions are abnormally higher only in respect to the given antigen (as compared with titers of serum from healthy controls), it proves that reaction has been caused by specific antibodies. On the other hand, if the serum reacts with many other antigens in titers higher than normal, this is a strong reason to suspect that the test is positive due to non-specific immunoglobulins. Unfortunately, such multi-antigen tests are not currently used to confirm the specific nature of a positive single-antigen tests. This is partially explainable by much higher technical complexity and cost of such verification tests, absence of commercial toolkits, as well as the lack of interest by mainstream immunology in this non-specific phenomena.

There are several reasons to assume that tests for "HIV-antibodies" are positive in AIDS-patients due to non-specific immunoglobulins. First, it is well known that total concentrations of non- specific immunoglobulins are much higher in almost all AIDS-patients than in healthy individuals. This condition, named hypergammaglobulinemia, is highly non-specific and observed in many diseases and abnormal states of organism. Thus, the principle of matched control is obviously violated in the aforementioned studies - not healthy individuals, but patients with hypergammaglobulinemia (but without AIDS) needed to be used as controls. Second, in many AIDS patients, titers of "HIV-antibodies" are low. Perhaps for these reasons information about titers is conspicuously absent in AIDS-literature. For example, in Russia, due to shortage of test systems the so called "pool-method" was frequently used - when blood from several individuals was mixed and tested. It was noted, that even such 2-8 fold dilution of the serum, may have resulted in a false negative test [8]. Thus, titers of putative "HIV-antibodies" in some AIDS patients are about 1:2 - 1:8. In immunology such low titers are usually not considered as significant at all [9] **. Third, AIDS patients and individuals from groups at high risk of AIDS are known to be seropositive in respect to many other antigens (e.g. hepatitis-B virus, EBV, etc.). Even though this is usually interpreted as a sign of infection by these pathogens, it is also well explainable by non-specific reactivity of the serum of these individuals [3].

Non-specific reactivity should not be confounded with cross-reactivity [3]. Cross-reactivity is a specific phenomenon, well understood in immunology. Even though cross-reacting antigens differ, they share common determinants, and reaction is specific in respect to these determinants. Normally only a small proportion of antigens cross-react to antiserum against a given antigen. In contrast to cross-reactions, neither mechanisms of production nor properties of non-specific immunoglobulins are understood in modern immunology. Textbooks of immunology are either silent or say only a few words about their existence. It is also rarely mentioned in the textbooks, that only a part, maximum 20-30 percent, of the immunoglobulins produced by B-cells in response to an antigen are capable of binding specifically to the antigen; the other 70-80% of the immunoglobulins are non-specific [10]. A hypothesis has been advanced that the affinity of non-specific immunoglobulins increases radically if the B-lymphocytes are over-stimulated and that just this effect leads to positive tests for HIV-antibodies [3].

The problem of non-specific immunoglobulins is exacerbated in the tests which are based on "sandwich" principle (as in ELISA and WB). In these test-systems, the antigen (e.g. "HIV- antigen") is attached to a surface and forms the first layer in the "sandwich". After exposure to the tested serum, immunoglobulins from the serum bind to the antigen and form the second layer in the "sandwich". To detect these immunoglobulins and estimate their quantity the two-layer sandwich is subject to one more procedure - exposure to antibodies against human immunoglobulins (which are obtained from laboratory animals immunized by human immunoglobulins). These animal antibodies bind to the human immunoglobulins and form the third layer of the sandwich. Only the amount of the animal antibodies bound to human immunoglobulins, not the quantity of the human immunoglobulins themselves, is being measured in test-systems of this sort [9]. It is tacitly postulated that affinity (ability to bind) of the animal antibodies to human immunoglobulins is about the same for all individuals and, hence, the amount of the animal antibodies bound is simply proportional to the amount of human immunoglobulins. But this is not the case if non-specific immunoglobulins from some individuals are capable of binding more strongly to various substances than immunoglobulins from healthy controls. Let us say, for example, that non-specific affinity of non-specific immunoglobulins increased 3 times in respect to various proteins, including both "HIV-antigens" and animal antibodies. Then, the number of molecules of human non-specific immunoglobulins bound per one molecule of the antigen is 3 times higher. After exposure to animal antibodies, 3 times higher number of molecules of the animal antibodies will be bound per one molecule of human immunoglobulins. Thus, the total amount of animal antibodies will be 9 times (3 multiplied by 3) higher, not 3 times. Hence, even a moderate increase in non- specific affinity of immunoglobulins may lead to radical increase in the titers and, hence, to HIV-seropositivity.

3. What increases the levels of non-specific immunoglobulins

Given that elevated levels of non-specific immunoglobulins and their increased affinity may lead to positive tests for "HIV-antibodies" it is reasonable to consider the causes of such conditions. It is widely accepted that hypergammaglobulinemia (which is typical to AIDS and many other conditions) results from polyclonal activation of B-lymphocytes caused by intensive stimulation by multiple foreign antigens. Individuals in groups with high risk of AIDS are exposed with abnormal frequency to such multiple antigens [1]: multiple infections, including STD and AIDS-defining opportunistic infections, anal reception of semen, contaminants of injected recreational drugs, foreign blood received either in course of sharing syringes for injection of such drugs or as transfusions, contaminants of the blood factors received by hemophiliacs as well as these factors themselves. Thus, the significantly higher frequency of positive tests for "HIV-antibodies" observed in the groups with high risk of AIDS is highly likely to be nothing but an indicator of such over-stimulation by multiple foreign antigens and, in many cases, an indicator of some diseases. Nevertheless, there are no factual reasons to consider the antigen overload itself as a life-threatening factor.

Along with the above mentioned factors, one more factor of antigen overload deserves closer attention - prolonged use of broad spectrum antibiotics. Such antibiotic abuse is closely associated with high promiscuity (frequent change of sexual partners): antibiotics used to treat frequent STDs as well as permanent prophylaxis of STDs (a fashion popular among promiscuous individuals). Moreover, permanent use of broad spectrum antibiotics is prescribed to many HIV-seropositive individuals and to most AIDS-patients as an apparent prophylaxis against opportunistic infections. Antibiotics cause antigen overload indirectly. These drugs suppress the friendly bacterial flora of the gut. These flora are of vital importance for digestion of food as well as for stifling various opportunistic pathogenic microorganisms. Suppression of the friendly flora of the gut by antibiotics results in serious problems with digestion of food and the development of opportunistic intestinal infections [14]. Such intestinal abnormalities frequently cause increased permeability of the gut walls ("leaky gut syndromes") [15]. Proteins are essential parts of our diet, and they are very powerful foreign antigens. Why don't they cause antigen overload in healthy individuals? Normally, proteins are digested into short fragments which are not antigens (cannot induce immune response), and only these non-antigenic short fragments permeate the gut walls and run into the blood stream. Abnormally high permeability of the gut walls makes it possible for molecules of proteins themselves to run into the blood stream and to become a powerful factor of antigen overload. This mechanism provides a plausible explanation for the epidemiological association between promiscuity, diagnosis of AIDS, and HIV-seropositivity, mediated by a common factor - antibiotic abuse. It also explains the unusually high rate of HIV-seropositivity in Africa, where intestinal infections are rampant.

Besides the role of foreign antigens, there is another plausible hypothesis advanced; it holds that both typical signs of AIDS - hyperactivation of B-cells and T4-lymphocytopenia - are intrinsic features of the classical stress-syndrome [11]. Stress-syndrome is a highly non-specific reaction of the organism to various adverse factors: diseases, intoxication, psychological trauma, etc. This reaction is mediated by elevated concentrations of corticosteroids ("stress-hormones"), and it may be induced by direct injection of corticosteroids. (Incidentally, corticosteroids are frequently used to treat inflammatory conditions in AIDS-patients.) If this hypothesis is combined with the aforementioned one (that hyperactivation of B-cells results in increased affinity of non-specific immunoglobulins), it provides a coherent explanation of why people with severe opportunistic infections (named AIDS) usually demonstrate T4-lymphocytopenia and HIV-seropositivity.

4. HIV and mortality in Africa: another look at the facts

In a study conducted in a rural population of Uganda (Lancet 1994, 343, 1021-23), about 10,000 individuals were tested for "HIV-antibodies". In those aged 13-44 years, 9.6% were found HIV- seropositive. During follow up, mortality was estimated as 96/1000 man-years (=96 persons out of 1000 in 1 year) in the HIV-positive group, and as only 1.4/1000 m.-y. in the HIV-negative group. Thus, mortality in HIV-seropositives was 60 times higher than in their HIV-negative counterparts. At first sight, these results seem to be a reliable proof for a causal role of HIV in AIDS, specificity of HIV-tests, and reality of HIV. For this reasons these results are frequently referred to by proponents of the HIV-AIDS theory (see for example [12,13]).

Let us look at the data from another standpoint, and consider an alternative hypothesis - that a positive "HIV-test" is only a non-specific marker of various infectious diseases. Such a "marker-effect" is likely to be caused by the elevated concentrations of non-specific immunoglobulins and an increase in their non-specific affinity associated with infectious diseases, especially multiple infections and intestinal ones (see section 4). Such diseases are known to be the main cause of mortality in this region, at least in relatively young ages. If HIV-seropositivity is actually only a marker of these diseases, most sick individuals in this population have to fall into the HIV- seropositive group. Hence, mortality in the HIV-seronegative group has to be much lower than the usual mortality rate in this region. On the other hand, if HIV-tests actually detect a new pathogen (HIV) and HIV causes additional mortality (as the mainstream AIDS science holds), mortality in the HIV-negative group should not decrease in the course of the HIV-epidemic. Thus, comparison of mortality in the HIV-negative group with its usual rate, observed before the hypothetical HIV-epidemic, can easily discriminate between the two hypotheses.

What is the usual mortality in this population? Even though reliable information about mortality in Uganda is absent, it is well known that a great proportion of population there usually die from various diseases at relatively young ages, as was the case long before the hypothetical HIV-epidemic. Is a mortality rate of 1.4/1000 in the HIV-negative group compatible with such information? The mortality rate of HIV-negative Ugandans at age 13-44 is even lower than mortality in the USA observed in the pre-AIDS era; in 1980, 157,685 deaths were registered in the USA at ages 15-44, and the population of this age group was 105,203,377. This gives a general mortality rate 1.5/1000. It is unreasonable to believe that the usual mortality in a rural population of Uganda is about the same as in the USA - one of the most prosperous countries in the world [16]. It is not compatible with the reality that a great proportion of Africans die and died young. Thus, mortality in the HIV-negative group (1.4/1000 m-y) is significantly lower than the usual mortality in this region. In other words the "HIV-test" selects a great proportion of individuals who would die regardless of the hypothetical "HIV-epidemic". This is in perfect agreement with the "HIV-is-only-a-marker" hypotheses.

Proponents of the HIV-AIDS theory [12] insist that the 9.3/1000 m-y mortality in the 13-44 age group at large is significantly higher than in other parts of the country, and this cannot be explained by causes other than HIV. Such argumentation is flawed - simply because the region was selected for this study because of its higher mortality than in other regions of Uganda. There are many other possible causes for the increase in morbidity and mortality from infectious diseases in some areas of an African country. Irrespective of the actual causes of this increase, both hypotheses predict much higher mortality in the HIV-seropositive group than in the HIV- negative one, and the causes of this difference cannot be discriminated by either hypotheses. Nevertheless, mainstream AIDS-scientists try to present this difference as a proof of the official HIV-causes- AIDS hypothesis. For some reasons, they "forget" to pay attention to the mortality rate in the HIV-negative group, which is obviously lower than the usual rate in this region - in perfect agreement with the "HIV-is-only-a-marker" hypothesis and contradicting the "HIV-causes-AIDS" one.

5. Other explanations for correlation between HIV-seropositivity and AIDS

The central goal of this summary is to show that there is no proof that a positive test for HIV-antibodies is caused by any specific antibodies, and that non-specific immunoglobulins are highly likely to be the actual cause of HIV-seropositivity. Let us imagine if it were shown experimentally that HIV-seropositivity is caused by specific antibodies - that is, blood serum from HIV-seropositive individuals reacts (in significantly higher titers than serum from healthy controls) only with the "HIV-proteins", but not with any other antigens. Surely, this would refute the hypothesis described here. Would such refutation be a proof that HIV-seropositivity is actually caused by HIV?

The main problem with the official HIV-causes-AIDS theory is that it has never been shown that "HIV-proteins" are related to a virus. The only thing known for sure is that these proteins are produced by human lymphocytes in certain conditions in vitro (in a test tube). To the same extent, they may be produced by the lymphocytes in vivo (in living organism). The "HIV-proteins" are likely to be of cellular (endogenous) nature [1] - that is, to be encoded in the human genome by normally inactive genes ("inactive gene" means that the protein encoded by this gene is not produced by the cell). It is well known that only a small proportion of genes in the human genome are active, and different sets of genes are active in different types of cells (even though the genome is the same for all cells of a given organism). Even in cells of the same type some genes can be switched on (or off) if conditions change. The mechanisms which switch genes on and off are poorly understood in modern biology. If in some abnormal conditions lymphocytes start to produce the "HIV-proteins" (the corresponding genes are switched on), these proteins will be "foreign" for the immune system and specific antibodies will be produced against these proteins. Naturally, blood serum of such individuals will yield specific reaction to the "HIV-proteins". In other words, specific antibodies against "HIV-proteins" may be only a marker that corresponding genes have switched on due to some metabolic changes. Thus, existence of HIV cannot be proven by immunochemical and serological methods - irrespective of whether HIV-seropositivity is caused by non-specific immunoglobulins or by specific antibodies.

Even if it were proven rigorously that HIV exists as an exogenous transmissible agent (this has never been done [1-4]) and that HIV-seropositivity is caused by HIV-infection, it still cannot prove that HIV is the cause of AIDS. Correlation between HIV-infection and AIDS-defining diseases is equally explainable by the "HIV-is-a-marker" hypotheses, which hold that HIV is a benign passenger virus [17] and can easily infect only individuals with some deviations from normal health status, thus, being only a marker of such deviations. In this case, morbidity and mortality may be much higher in HIV-positive individuals than in their HIV-negative counterparts, but not because of HIV-infection. Critical reevaluation of the studies carried out in Africa (see section 5) demonstrates that the results support the "HIV-is-only-a-marker" hypotheses, and contradict the HIV-causes-AIDS one irrespective of the actual causes of HIV-seropositivity.

Conclusions

Specificity of antibodies cannot be established in serological studies with one antigen: it is necessary to prove that titers of the antigen-antibody reaction are significantly higher (than in healthy controls) only for this antigen, but not in respect to other antigens. Given that such multi- antigen serological studies have never been carried out, increase in non-specific affinity of immunoglobulins is the most likely cause of HIV-seropositivity. The problem is exacerbated by the use of "sandwich" tests (like ELISA and WB) - because they are abnormally sensitive to any increase in affinity of non-specific immunoglobulins. Besides the non-specific immunoglobulins, there are several other mechanisms which can lead to correlation between HIV-seropositivity and diseases, while not being compatible with the official "HIV-causes-AIDS" hypothesis. The main flaw of the mainstream AIDS-science is that no experimental or epidemiological studies have been designed and carried out to rule out such alternative explanations. There are no reasons to consider HIV-seropositivity as a reliable marker of a deadly disease. The main danger of HIV- seropositivity is of iatrogenic (caused by medicine) nature: such individuals are at high risk of being administered abnormally severe and prolonged "prophylactic" treatment (antibiotics, antiretrovirals). This iatrogenic effect is a direct consequence of the uncritical acceptance of the HIV-causes-AIDS theory.

Vladimir Koliadin Ph.D. is a Senior Research Scientist at The State Aerospace University in the Ukraine and a member of the American Mathematical Society.

Endnotes

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Is a Positive Western Blot Proof of HIV Infection?
Papadopulos-Eleopulos et al, Bio/Technology 11, pp. 697-707, June 1993
http://www.virusmyth.com/aids/data/epwbtest.htm

[Abstract] It is currently accepted that a positive Western blot (WB) HIV antibody test is synonymous with HIVinfection and the attendant risk of developing and dying from AIDS. In this communication we present a critical evaluation of the presently available data on HIV isolation and antibody testing. The available evidence indicates that: (I) the antibody tests are not standardised; (II) the antibody tests are not reproducible; (III) the WB proteins (bands) which are considered to be coded by the HIV genome and to be specific to HIV may not be coded by the HIV genome and may in fact represent normal cellular proteins; (IV) even if the proteins are specific to HIV, because no gold standard has been used and may not even exist to determine specificity, a positive WB may represent nothing more than cross-reactivity with the many non-HIV antibodies present in AIDS patients and those at risk, and thus be unrelated to the presence of HIV. We conclude that the use of the HIV antibody tests as a diagnostic and epidemiological tool for HIV infection needs to be reappraised.

 

** In immunochemical methods, which provide mainly qualitative answers "yes-no", the following method is used to obtain semi-quantitative results. The samples are being diluted until the results of the test switch from "yes" (positive) to "no" (negative). Maximal dilution, for which the result is still "yes" is named "titer of the reaction". For example, the titer 1:128 means that after dilution 128 times (i.e. 7 consecutive 2-fold dilutions) the sample still was positive. Surely, the greater the magnitude of the titer, the greater the strength of reaction. Normally, titers vary from experiment to experiment by 2-4 or even 8 times for various reasons. So, the titer 1:2 or even 1:8 is not considered as significant enough to say that the sample is really positive.

In Russia, it was found occasionally that even relatively small dilution 3-8 times (when samples from 3-8 individuals are pooled together) often lead to negative results of ELISA, when one sample of the several ones was positive (if tested separately - not in the pooled). Technically this means that titers of [antigen-antibody] reaction was quite low - < 1:3 -1:8 - lower than standards of practical immunochemistry require.

 

References

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