The Patent
Antiviral composition
1. A polysaccharide derivative containing at least one sulfate group and at
least one alkylsulfate group.
2. The compound of claim 1, wherein the polysaccharide is selected from the
group consisting of dextrin, dextran, and cyclodextrin.
3. The compound of claim 1, wherein the at least one alkylsulfate group is
selected from the group consisting of methylsulfate, ethylsulfate and
propylsulfate.
4. A pharmaceutical composition unit dosage form comprising an active agent,
present in an amount sufficient to provide antiviral activity, said active agent
selected from the group consisting of alkylsulfate derivative of sulfated
dextrin and alkylsulfate derivative of sulfated dextran, and at least one
excipient.
5. The pharmaceutical composition unit dosage form of claim 4, wherein the
active agent is an ethyl sulfate derivative.
6. The pharmaceutical composition unit dosage form of claim 4, wherein the
active agent is an ethyl sulfate derivative.
7. The pharmaceutical composition unit dosage form of claim 4, wherein the
active agent is a propyl sulfate derivative.
8. The pharmaceutical composition of claim 4, wherein the antiviral activity is
provided against a virus selected from the group consisting of HIV, herpes
viruses such as cytomegalovirus and herpes simplex, hepatitis agents, and the
papilloma virus.
9. A method of treating a viral infection comprising administering to a patient
in need thereof a therapeutically effective amount of an active agent comprising
an alkylsulfate derivative of a sulfated dextrin starting material having a
molecular weight of at least 3,000, wherein the sulfated dextrin starting
material is sulfonated to form the alklysulfate derivative of sulfated dextrin,
wherein the range of sulfonation of the alkylsulfate derivative of sulfated
dextrin is between 12 to 21%, wherein the sulfonation occurs in clusters of
alkylsulfate groups and sulfate groups present on the branch point structures of
the sulfated dextrin, and further wherein the ratio of alkylsulfate groups to
sulfate groups is about 1 to 2.
10. The method of claim 9, wherein the active agent is an methyl sulfate
derivative.
11. The method of claim 9, wherein the active agent is an ethyl sulfate
derivative.
12. The method of claim 9, wherein the active agent is an propyl sulfate
derivative.
13. The method of claim 9, wherein the antiviral activity is provided against a
virus selected from the group consisting of HIV, herpes viruses such as
cytomegalovirus and herpes simplex, hepatitis agents, and the papilloma virus.
14. The method of claim 9, wherein the administering is selected from the group
consisting of oral administering, topical administering, subcutaneous
administering, administering by muscular injection, administering by
intraperitoneal injection and administering by intravenous injection.
15. The method of claim 9, wherein the administering occurs in combination with
administering of another agent.
16. A method of preventing viral transmission, comprising applying to a patient
a therapeutically effective amount of an active agent comprising an alkylsulfate
derivative of sulfated dextrin and alkylsulfate derivative of sulfated dextran
as a topical formulation, wherein the alkylsulfate derivative of sulfate dextrin
is prepared using a dextrin starting material having a molecular weight of at
least 3,000.
17. The method of claim 16, wherein the active agent is a methyl sulfate
derivative.
18. The method of claim 16, wherein the active agent is an ethyl sulfate
derivative.
19. The method of claim 16, wherein the active agent is a propyl sulfate
derivative.
20. The method of claim 16, wherein the viral transmission prevented is the
transmission of a virus selected from the group consisting of HIV, herpes
viruses, hepatitis agents, and the papilloma virus.
21. A method of eliminating virus from entities selected from the group
consisting of blood, blood products, organs and whole body preparations,
comprising combining the entities with an effective amount of an active agent
selected from the group consisting of alkylsulfate derivative of sulfated
dextrin and alkylsulfate derivative of sulfated dextran as a topical
formulation.
22. The method of claim 21, wherein the active agent is a methyl sulfate
dertivative.
23. The method of claim 21, wherein the active agent is an ethyl sulfate
derivative.
24. The method of claim 21, wherein the active agent is a propyl sulfate
derivative.
25. The method of claim 21, wherein the virus eliminated is selected from the
group consisting of HIV, herpes viruses, hepatitis agents, and the papilloma
virus.
26. The method of claim 9, wherein the sulfated dextrin staring material is
sulfonated using compounds selected from the group consisting of a pyridine
sulfurtrioxide complex, chlorosulfonic acid and methanesulfonyl chloride.
27. The method of claim 16, wherein the alkylsulfate derivative of sulfate
dextrin is prepared from the dextrin starting material using compounds selected
from the group consisting of a pyridine sulfurtrioxide complex, chlorosulfonic
acid and methanesulfonyl chloride.
Chemical compounds, being the alkyl sulfate of sulfated saccharides,
particularly, dextrin, dextran, and cyclodextrin, and pharmaceutical
compositions containing these compounds. The compounds of the invention provide
antiviral activity, particularly in the treatment and prevention of
sexually-transmitted diseases. Methods of treating viral infection and
preventing viral transmission include administration include administration of
the compounds of the invention orally, topically, subcutaneously, by muscular
injection, by intraperitoneal injection and by intravenous injection.
Agent: The Webb Law Firm, P.C. - Pittsburgh, PA, US
Inventor: Roger Hershline,
Charlotte, NC, US
Class: 514058000 (USPTO), A61K031/724 (Intl Class)
20050209189 - Antiviral composition
Full Patent Description
CROSS REFERENCE TO RELATED APPLICATIONS
[0001] This application claims the benefit of U.S. patent application Ser. No.
10/157,787, filed May 29, 2002, which claims priority to U.S. patent application
Ser. No. 10/092,021, filed Mar. 6, 2002, which claims priority to U.S.
Provisional Patent Application Nos. 60/288,032, filed May 2, 2001; and
60/273,724, filed Mar. 6, 2001, all of which are incorporated herein by
reference.
BACKGROUND OF THE INVENTION
[0002] 1. Field of the Invention
[0003] The present invention relates to the production of the alkyl sulfate of
sulfated dextrin, the production of the alkyl sulfate of sulfated dextran, and
to the use of these compounds to provide antiviral activity, particularly in the
treatment and prevention of sexually-transmitted diseases.
[0004] 2. Description of Related Art
[0005] Compounds exhibiting activity against viruses may function by a number of
mechanisms: they may kill or disable the disease pathogens, they may inhibit the
entry of the pathogen into cells, or they may prevent replication of the
pathogen once it has entered a cell. All of these mechanisms are being studied
to prevent and treat viral infection, including those resulting in diseases that
can be sexually transmitted, such as Acquired Immunodeficiency Disease Syndrome
(AIDS).
[0006] The generally accepted theory is that AIDS is caused by the Human
Immunodeficiency Virus (HIV). There are two different versions of HIV: HIV-1 and
HIV-2. These viruses are believed, on the basis of their genetic sequences, to
have evolved from the Simian Immunodeficiency Virus (SIV), with HIV-2 being much
more similar to SIV. Several years after the initial HIV infection, the immune
system is weakened to the point where opportunistic infections occur, resulting
in the syndrome of AIDS.
[0007] Research has revealed a great deal of valuable medical, scientific, and
public health information about HIV and AIDS. HIV molecules whose structures are
known include reverse transcriptase (RT), proteases of HIV-1 and HIV-2, the
catalytic domain of HIV integrase (INT), the HIV matrix protein, the HIV capsid
protein and several fragments of CD4. HIV macromolecules whose structures are
being investigated include the surface glycoproteins (gp160, gp120, gp41), and
the regulatory proteins (tat, rev, vpr, tar).
[0008] The ways in which HIV can be transmitted have been clearly identified.
HIV is spread by sexual contact with an infected person, by sharing needles
and/or syringes (primarily for drug injection) with someone who is infected, or
through transfusions of infected blood or blood clotting factors. Babies born to
HIV-infected women may become infected before or during birth or through
breast-feeding after birth. In the health care setting, workers have been
infected with HIV after being stuck with needles containing HIV-infected blood
or, less frequently, after infected blood gets into a worker's open cut or a
mucous membrane (for example, the eyes or inside of the nose). HIV is found in
varying concentrations or amounts in blood, semen, vaginal fluid, breast milk,
saliva, and tears.
[0009] In recent years, medical science has made great progress in the ability
to successfully treat the opportunistic infections associated with HIV
infection. Wider use of medications for preventing tuberculosis, Pneumocystis
carinii pneumonia (PCP), toxoplasmosis, and Mycobacterium avium complex (MAC),
for example, has helped reduce the number of people with HIV who develop serious
illness and die from AIDS.
[0010] Also, several classes of compounds have been federally approved to treat
HIV infection. These include nucleoside RT inhibitors (AZT, ddI, ddC, d4T and
3TC), non-nucleoside RT inhibitors (alpha-APA, TSAO, costatolide, TIBO, UC10),
protease inhibitors (indinavir, saquinavir, KNI 272), attachment inhibitors
(sulfate polysaccharides, sulfonated dyes) and neutralizing antibodies.
Combinational therapy with these drugs seems to produce the best results,
reducing the level of HIV particles circulating in the blood (viral load) to
very low levels in many individuals.
[0011] Though treatment results using these drugs have been encouraging, the
virus is not eliminated, these drugs do not work for all people, there are
adverse interactions with other medications, toxicity to the drugs is
problematic, dosing protocols are complex, resistance to treatment develops, and
expense is extremely high. Furthermore, long-term effectiveness and safety are
completely unknown. Clearly, there remains a need for new therapies.
[0012] Attempts to develop a vaccine have not been successful to this point.
[0013] Testing facilities perform in vitro analyses to identify compounds with
antiviral activity. Therapeutic indices of active compounds are evaluated using
several viral strains. Many viruses are routinely available for the testing of
compounds for antiviral activity in viruses other than HIV, including the
herpesviruses HSV-1, HSV-2, HCMV, VZV and EBV; the respiratory viruses Flu A,
Flu B, RSV, Paraflu 3 and Ad5; measles and hepatitis B virus. Anti-HIV assays
are routinely performed in established cell culture lines. Recently fresh human
peripheral blood lymphocytes (PBMCs) have been introduced as test media.
[0014] Assays measure the ability of compounds to directly inactivate the HIV
virus and inhibit HIV-induced cell killing through numerous enzyme-inhibiting
mechanisms (Reverse Transcriptase, RNaseH, Integrase, Protease, Tat, Rev and Nef),
by preventing attachment and internalization (inhibit gp120-CD4 interaction) or
by inhibiting regulatory protein expression, or by inhibiting maturation and
budding, or by preventing Syncytical formation. Toxicity of the test compounds
to host cells is also measured. It is generally accepted that if the test
compound is highly toxic to cells, then it will have little value despite
anti-HIV activity.
[0015] Infectious virus levels are measured by viral titers, quantitation of p24
(a viral protein found to be proportional to viral concentration) or measurement
of the activity of the viral enzymes.
[0016] Several parameters are routinely varied to more completely understand the
potential of a particular drug. The concentration of a drug is varied to
calculate the ED50 (Effective Dose at 50% inhibition), LD50 (Lethal Dose at 50%
cell death), and TI50 (Therapeutic Index, which is the Effective Dose divided by
the Lethal Dose).
[0017] The concentration of the initial viral load is varied in the cell system
used for testing to help determine drug potency. The time of drug addition to
the cell system, either pre- or post-infection, is varied to identify strengths
and weaknesses in the drug mechanism of action. Another test is to add the drug
to the cell system and then wash it away before infection. This gives insight
into cell-drug mechanisms of action. Topical assays test drugs which may be of
use as preventive barriers. Both viral killing and cellular toxicity are
measured in these assays.
[0018] Active anti-HIV compounds will likely be used in combination with other
anti-HIV agents, with agents that inhibit opportunistic agents, or with other
therapies. Therefore, the compounds are tested with all known useful drugs to
determine beneficial synergistic effects or possible harmful combinatorial
toxicity.
[0019] Drugs that prove to be successful in in vitro testing are selected for
animal testing. Several animal models have proven to be helpful including
systems using the mouse, cat, and rhesus macaque. The test compound and virus
can be administered by a variety of methods and routes in addition to the
variables discussed above. Animal mucosal models of HIV transmission may be
useful for the evaluation of possible therapeutic agents. Test compounds that
may have limited effectiveness in fully developed HIV may be effective at the
time of initial infection. Models are useful in exploring this possibility.
Animal models traditionally have been used for the pre-clinical evaluation of
lead compounds to determine mechanism of action, distribution, toxicity, and
efficacy.
[0020] Antiviral compounds are also being investigated for use as microbicides.
A "microbicide" is any substance that can substantially reduce transmission of
sexually transmitted infections (STIs) when applied either in the vagina or
rectum. Target viruses include herpes viruses such as cytomegalovirus and herpes
simplex, hepatitis agents, and the papilloma virus. Proposed forms for
microbicides include gels, creams, suppositories, films, and sponges or vaginal
rings that slowly releases the active ingredient over time. Microbicides are not
currently available commercially, but a number of compounds, including
nonoxynol-9, cellulose sulfate, carrageenan, cyanovirin, the sulfated
polysaccharide PRO2000 and dextrin sulfate, are currently being evaluated.
Dextrin sulfate has been found to have a high level of toxicity. Nonoxynol-9 has
been found to cause inflammation of mucosa that may actually enhance the chance
of infection. There remains a need for a proven effective nonirritant antiviral
compound of low toxicity for use as a microbicide.
[0021] Polysulfonated polysaccharides (PSP) have been previously proposed to be
used to treat HIV infection. The most studied include curdlan sulfate (CDS),
dextrin sulfate, dextran sulfate (DS), and heparin sulfate. Many of these,
including dextran sulfate, curdlan sulfate and dextrin 2-sulfate, have been
studied in human trials. Many other naturally occurring isolated sulfates have
been shown to inhibit the AIDS virus. Smaller non-polymeric sulfated sugar based
compounds included pentosan sulfate and glucosamine sulfate.
[0022] Though the results indicate that sulfates are a viable lead for the
development of an anti-HIV drug, several problems remain. Firstly, the large
anionic structures of the PSPs show very poor absorption or no absorption from
oral administration. Secondly, when PSP's are given intravenously the toxic
effects of seriously decreasing the amount of platelets and decreasing the
ability of blood to clot become limiting factors. Oral administration is also
related to serious gastrointestinal toxic effects including the possible
development of cancers demonstrated in rodents. Furthermore, there is no
protection of the compounds from sulfatase enzymes which rapidly degrade these
compounds and shorten the half-life.
[0023] The use of dextrin-2 sulfate as an anti-HIV compound versus generically
sulfated dextrin (that is sulfates at any or all of the 2, 3 or 6 positions of
the glucose units) has also been proposed. The use of dextrin-2 sulfate is an
attempt to decrease toxicity while maintaining anti-HIV activity. Recent
attempts to administer dextrin-2 sulfate by intra-peritoneal administration
(that is, infusion into the body cavity by a catheter passing through the
abdominal wall as done in peritoneal dialysis) shows some promise in decreasing
HIV infection while decreasing intravenous-type side effects. However, the
intra-peritoneal method introduces extremely little if any drug to the systemic
circulation and relies upon the lymphatic circulation to expose circulating HIV
infected white blood cells to the drug as they pass through the peritoneal
cavity. Evaluation of dextrin 2-sulfate shows that the anti-platelet effect and
anti-coagulant effect persists and there is no attempt at chemical inhibition of
the hydrolysis of the drug by hydrolyzing enzymes. Consequently, dextrin
2-sulfate has not been shown to provide significant advantages over dextrin
sulfate.
[0024] Accordingly, there remains a need to identify and synthesize a compound
with minimized toxicity, providing antiviral activity including, but not limited
to, microbicidal activity. There remains a need for a pharmaceutical composition
incorporating this compound, and for methods of treatment, inhibition of viral
transmission, and elimination of virus in blood, blood products, organs and
whole body preparations incorporating this compound.
SUMMARY OF THE INVENTION
[0025] The present invention is directed to a new class of compounds, methods
for their synthesis, and to the use of these compounds in providing antiviral
activity. This class of compounds is produced by alkylsulfation (alkylsulfonation)
and sulfation (sulfonation) of dextrin or dextran. The reaction used introduces
aliphatic alkyl groups and sulfur groups onto a carbohydrate or polysaccharide.
This reaction randomly replaces the reactive hydrogen atoms with a methylsulfate
group or a sulfate group and allows for a combinatorial production of sulfate
and methylsulfate substitution of dextrin or dextran. The variables of this
reaction that can be controlled include the choice of dextrin or dextran as a
reactant, the polymeric size of the starting material, the degree of total
methylsulfation and sulfation, the degree of methylsulfation and sulfation per
saccharide, and position of methylsulfation and sulfation (sulfonation) and the
character of the counter ion. Control of these variables, along with the
polymeric size of the starting material and degree of hydrolysis during the
reaction or work-up, produces a wide range of polymeric compounds. These new
compounds are distinctly different from other compounds introduced for anti-HIV
therapy. These compounds have a unique synthesis, unique chemical properties and
a unique pattern of activity against HIV. Use of these compounds overcomes the
absorption obstacles, toxicity obstacles, and efficacy obstacles presented by
prior art compounds while retaining the anti-HIV properties of sulfated
saccharides. Use of the compounds of the present invention, incorporating alkyl
sulfonate groups, embodies the realization that these obstacles are related to
the linear sulfated structures and the non-attenuated high degree of anionicity
characteristic of these sulfated compounds, and the lack of the presence of an
inhibitor to enzymatic sulfate hydrolysis.
[0026] The invention introduces four important changes. First, the crucial
structural element required for anti-HIV activity is recognized to be the
cluster of sulfate groups presented on the branch point structures. Second, the
structural element of toxic side effects is recognized as the sulfate groups on
the linear portions. Elimination of linear portions and amplification of branch
point sulfated structures decreases toxic side effects and increases therapeutic
effects. Third, introduction of the methylsulfate group in synergy with the
sulfate group increases efficacy by several possible mechanisms, including the
providing of an inhibitor to sulfate hydrolyzing enzymes, the attenuation of the
large negative charge and the proposed increase in oral, systemic and cellular
absorption and efficacy. Finally, the number of sulfated structures or
combinations of structures provides variable sites for binding and enzyme
inhibition.
[0027] The antiviral activity of the compounds of the present invention is
explained here in relation to, but is not limited to, the Human Immunodeficiency
Virus (HIV). The generally accepted theory is that Acquired Immunodeficiency
Disease Syndrome (AIDS) is caused by the Human Immunodeficiency Virus (HIV) and
that the prevention of the reproduction of HIV will prevent AIDS. The
reproduction of the virus relies on the function of the reverse transcriptase
enzyme (RT). RT function requires the binding protein Trans Activating
Transcriptor (TAT). The present invention prevents the reproduction of HIV by
binding with the TAT protein and preventing the proper function of RT.
[0028] The comparatively low toxicity and comparative absence of detrimental
effects on body tissue allow the use of the compounds of the present invention
in a number of applications calling for compounds exhibiting antiviral activity.
The compounds may be used directly, alone or in combination with other therapy,
as an antiviral or anti-HIV drug. The compounds of the present invention may
also be used in preventative treatments for HIV or other viruses. Routes of
administration for these uses include oral and topical administration, and sub-cutaneous,
muscular, intraperitoneal or intravenous injection. The compounds of the present
invention may be used in bound and unbound form to eliminate HIV or other
viruses from blood products during dialysis of organ or whole body preparations.
They may also be used alone or in combination in cell culture systems or organ
preservation systems to destroy or prevent HIV or other viral growth.
BRIEF DESCRIPTION OF THE DRAWINGS
[0029] FIG. 1 is a pictorial illustration of dextrin;
[0030] FIG. 2 is a pictorial illustration of a limit dextran;
[0031] FIG. 3 is one exemplary chemical structure for polysulfated
polymethylsulfated dextrin;
[0032] FIG. 4 shows Structure 1 of a polysulfated polymethylsulfated dextrin
compound linked to a branch point glucose molecule with an .alpha. 1.fwdarw.6
linkage;
[0033] FIG. 5 shows Structure 2 of a polysulfated polymethylsulfated dextrin
compound linked to a branch point maltose molecule with an .alpha. 1.fwdarw.6
linkage;
[0034] FIG. 6 shows Structure 3 of a polysulfated polymethylsulfated dextrin
compound linked to a branch point maltose molecule with an .alpha. 1.fwdarw.6
linkage and linked to a branch point glucose molecule with an .alpha.1.fwdarw.4
linkage;
[0035] FIG. 7 shows Structure 4 shows a polysulfated polymethylsulfated dextrin
compound linked to a branch point glucose molecule with an .alpha.1.fwdarw.6
linkage and linked to a branch point glucose molecule with an .alpha. 1.fwdarw.4
linkage;
[0036] Table 1 lists the various chemical moieties that can be substituted on
carbons 2-4 and 6 of the different glucose molecules for Structure 1;
[0037] Table 2 lists the various chemical moieties that can be substituted on
carbons 2-4 and 6 of the different glucose molecules for Structure 2;
[0038] Table 3 lists the various chemical moieties that can be substituted on
carbons 2-4 and 6 of the different glucose molecules for Structure 3;
[0039] Table 4 lists the various chemical moieties that can be substituted on
carbons 2-4 and 6 of the different glucose molecules for Structure 4; and
[0040] Table 5 shows the resulting p24 values (pg/ml) as a measurement of HIV
concentration for the indicated concentrations of three separate efficacy tests.
DESCRIPTION OF THE PREFERRED EMBODIMENTS
[0041] The starting material for synthesis of the product of the present
invention is common corn starch or dextrin, pictorially illustrated in FIG. 1.
Dextrin is chemically characterized as a glucose polymer. The polymer consists
of linear chains having glucose units linked with alpha (1-4) glycocidic bonds.
Multiple linear chains are linked with alpha (1-6) glycosidic bonds along the
length of any other given linear chain. The resulting structure increases in
size as more glucose molecules are added increasing the length of the linear
chains and increasing the number of the branches. The group of glucose molecules
having both alpha (1-4) and alpha (1-6) glycosidic bonds is termed the branch
point or branch point structure.
[0042] Degradation of the starting dextrin with enzymes has been discussed in
the scientific literature. The process involves treatment of the dextrin with
starch-digesting enzymes called amylases. Beta-amylase is an exo-glycosidase
which hydrolyzes polysaccharides at alpha-(1-4) links from the non-reducing end
liberating two glucose units or maltose. The cleavage continues until the enzyme
encounters an alpha-(1-6) link and then stops. The branch point glucose
molecules will have either none or one glucose molecule remaining attached to
each of the exposed non-reducing number four carbons. This resulting highly
branched starch molecule is called a beta-limit dextrin. Alpha-amylase is an
endo-glycosidase which hydrolyzes polysaccharides at alpha-(1-4) links from the
reducing end. The enzyme requires a polymer of seven glucose molecules to attach
so the next glucose molecule can be cleaved. The alpha-amylase will not
hydrolyze alpha-(1-6) links and has decreased activity at alpha-(1-4) links
located next to the alpha-(1-6) links. However, the hydrolysis will occur
between two neighboring alpha-(1-6) branch points if the required number of
seven alpha-(1-4) links are present. Branch points are separated by about
twenty-five glucose molecules in starch amylopectin. Hydrolysis by alpha-amylase
would result in a branch point with short linear portions of seven to
twenty-five glucose molecules attached to the non-reducing carbon number four of
the branch point glucose molecules and a glucose polymer of zero to eighteen
(that is 25 minus 7) glucose molecules attached to the reducing carbon one of
the branch point glucose. This resulting collection of molecules is called an
alpha-limit dextrin. A representative pictorial illustration of a limit dextran
is shown in FIG. 2.
[0043] Exhaustive enzymolysis of the starch results in the production of pure
branch points or branch points with short linear segments of glucose alpha-(1-4)
polymers attached to the branch point. The branch point structures vary by the
number of glucose units and availability of substitution position. As a result
of the processes which produce the branch point structures, the number of
glucose units at the non-reducing end of the branch point will be necessarily
very short and contain either no extra glucose units or one unit in the most
commonly occurring situation, two glucose units as the next most common
situation and three glucose units in the least likely situation. The presence of
four or more glucose units at the non-reducing end of the branch point indicates
incomplete reaction hydrolysis. The length of glucose linear polymer at the
reducing end of the branch point will range from no extra glucose units to seven
glucose units in the most commonly occurring situation. Chain lengths of eight
to eighteen glucose units are possible but the abundance falls as the length
increases. The most preferred branch points have either none or one extra
glucose molecule at either of the non-reducing branch point carbon four
positions and a short polymer of eight or less glucose molecules at the reducing
carbon one of the branch point. A third method of obtaining branch point
structures, discussed in the scientific literature, is to synthesize the branch
point structures from individual glucose units.
[0044] There are two possible synthetic paths to obtain the branch point
polysulfated polymethylsulfated dextrin product starting with dextrin. The first
path involves enzymatic or chemical degradation of the starting material dextrin
into a structure which will expose the branch point structures followed by
chemical replacement of the hydroxyl groups with sulfate and methylsulfate
groups. The second path involves chemical replacement of the hydroxyl groups
with sulfate and methylsulfate groups as the first step, followed by enzymatic
or chemical degradation to eliminate non-branch point structures.
[0045] Chemical replacement of the hydroxyl groups with charged sulfate groups
and non-charged methylsulfate groups is performed by a simultaneous competitive
reaction of reagents such as chlorosulfonic acid, methylchlorolsulfonate, and a
sulfurtrioxide pyridine complex on the limit dextrin or branch point structure
starting material. This chemical replacement, however, can be performed in two
individual steps. Also, there are changes that can be made in the choice of
reagent or solvent. These changes may alter the purification techniques required
to obtain end product suitable for use in clinical studies.
[0046] The total sulfate composition of the polysulfate polymethysulfate dextrin
is about 12 to 21 percent sulfation. It is proposed that, because of the
increased reactivity of the sulfation reagent over the methylsulfation reagent,
the ratio of sulfate to methylsulfate will favor sulfate by about 2 to 1. It is
also proposed that the exposed or primary branch point carbon groups will have
the highest degree of sulfation. The secondary branch points, defined as the
second branch from the exposed surface, react at a decreased rate and are less
sulfated. Position 6 is the most exposed and the most highly susceptible to
substitution. Position 2 and position 3 are the least likely for sulfate
substitution and would be expected to be present in a low proportion. Position
4, if hydrolyzed, has a high probability of substitution.
[0047] To obtain active product with the least number of side effects the length
of linear chains should be minimized and the number of sulfate and methylsulfate
groups should be minimized. As the parameters are limited the potency of the
drug may decrease. The potency of sulfated polysaccharides has been shown to be
related to the degree of sulfation and size of the polymer. The minimum number
of glucose units with strategically located methylsulfate and sulfate groups is
the most preferred. For example, one methylsulfate group located at the carbon-6
position of the leading glucose unit and one sulfate group at the carbon-2
position of the base glucose of the branchpoint is a preferred arrangement.
[0048] The synthetic strategy is to ultimately obtain a collection of branch
point structures with varying amounts of combinatorial chemical alteration. The
chemical alteration is the replacement of the hydroxyl groups of the individual
glucose molecules in the branch point structure with either a negatively charged
sulfate groups accompanied with a suitable counter ion or a non-charged
methylsulfate group. The number of possible differing chemical structures is
large and is calculated from the variability of the branch point structure, the
number of charged versus non-charged sulfate groups on a particular branch point
structure, the position of the charged versus non-charged groups on the branch
point structure, and the nature of the counter ions. FIG. 3 shows one exemplary
chemical structure for the polysulfated polymethylsulfated dextrin compound of
the present invention. FIGS. 4-7 show four polysulfated polymethylsulfated
dextrin compounds, each one differing in their branch point structures. For
example, Structure 1 is a polysulfated polymethylsulfated dextrin compound
linked to a branch point glucose molecule with an .alpha. 1.fwdarw.6 linkage, as
shown in FIG. 4. Structure 2 is a polysulfated polymethylsulfated dextrin
compound linked to a branch point maltose molecule with an .alpha. 1.fwdarw.6
linkage, as shown in FIG. 5. Structure 3 is a polysulfated polymethylsulfated
dextrin compound linked to a branch point maltose molecule with an .alpha.
1.fwdarw.6 linkage and linked to a branch point glucose molecule with an .alpha.
1.fwdarw.4 linkage, as shown in FIG. 6. Structure 4 is a polysulfated
polymethylsulfated dextrin compound linked to a branch point glucose molecule
with an .alpha. 1.fwdarw.6 linkage and linked to a branch point glucose molecule
with an .alpha. 1.fwdarw.4 linkage, as shown in FIG. 7. Tables 1-4 list the
various chemical moieties that can be substituted on carbons 2-4 and 6 of the
different glucose molecules for Structures 1-4, respectively.
[0049] Applicant believes, without wishing to be bound by the statement, that
the alkylsulfate of limit dextrin contributes to the activity of the alkyl
sulfate of sulfated dextrin of the present invention.
[0050] The methylsulfate group and other alkylsulfate groups, such as
ethylsulfate or propylsulfate groups, may also be added to any other sulfates
that have been tested for antiviral activity, such as cyclodextrin sulfate and
other non-polymeric structures. The resulting compounds include saccharides
containing both sulfate and alkylsulfate groups. Dextrin, dextran and
cyclodextrin may serve as the saccharides.
[0051] Numerous mechanisms of action have been proposed for the observed
anti-HIV activity of the sulfated saccharides. These previously proposed
mechanisms of actions support the demonstrated anti-HIV activity of the
invention. In addition, unique mechanisms of action are proposed to explain the
function of the invention.
[0052] The large and highly negatively charged polymeric polysulfates are not
believed to be capable of entering the cell. The mechanism of action of these
large sulfates involve processes at the surface of the cell. These include the
prevention of viral absorption into the cell or prevention of budding of the
reproduced virus from the cell. As opposed to the linear binding array as
represented by dextran sulfate and curdlan sulfate, the invention places the
proposed active branch points, or alpha 1-6 gycosidic linkages, on the surface
of the molecule creating a three dimensional surface which enhances the binding
the invention and the proteins at the cell surface.
[0053] However, in the cellular based testing results presented of the proposed
compound, the virus was first placed in the cell before addition of the test
compound. Therefore, because the virus was already in the cell, reproduction
within the cell did not depend on entry. If the test compound simply prevented
the HIV particle from entering the cell then it should show no activity in this
type of assay. This is evidence that the mechanism of action is intracellular
which is different from the known mechanism of action of dextran sulfate.
[0054] Binding to internal enzymes of the virus has to be considered as a
possible mechanism. Experiments with HIV inhibition demonstrate that viral
reproduction is inhibited by intracellular mechanisms. The route of absorption
of a compound of the present invention may be enhanced because of the lipophilic
characteristics of the methylsulfate group. This lipophilic characteristic of
the compound may shield the electrostatic repulsion between the compound and the
outer wall of the cell so that the compound can pass into the interior of the
cell. Inhibition of intracellular reverse transcriptase or protease enzymes is
known to effectively inhibit viral reproduction. Other enzymes may also be
effected.
[0055] The TAT protein is a unique protein in that it plays both an
extracellular and intracellular role in viral reproduction. TAT binds with RT to
allow accelerated DNA synthesis and is thought to be the reason for the great
increase in viral load during active infection. This protein is manufactured in
large numbers and is released from the infected cell. The TAT protein then
enters uninfected cells awaiting the arrival of the virus. Once infected, the
newly functioning RT is able to immediately function at the accelerated level.
The binding of the sulfate group to an active site arginine on the TAT protein
is proposed to be the mechanism of inhibition. This proposed mechanism would
explain the ability of the invention to prevent systemic viral conversion during
the initial periods of infection.
[0056] The polysulfated polymethysulfate exhibits an increased antiviral
activity in comparison to dextrin sulfate. A proposed explanation is that the
high concentrations of enzymes in the white blood cells called sulfatases, which
hydrolyze the sulfate group, inactivates polysulfated compounds. The
polymethylsulfate derivative of polysulfate dextrin retains activity, possibly
because the methylsulfate moiety acts as an inhibitor of the sulfatase enzyme.
This prevents drug decomposition or deactivation.
[0057] A number of routes of administration are suitable for the compounds of
the present invention. These compounds are included, for therapeutic evaluation,
in antiviral compositions containing excipients appropriate to the route of
administration. The route of administration of a drug may be oral, topical,
intra-peritoneal/-muscular/-cutaneous or intravenous. The route used depends on
the ability to achieve therapeutic results along with minimization of side
effects and eventually compliance. As a drug of the nature of the drug of the
present invention is developed, the optimum goal is to develop an oral dosing
medication.
[0058] The early stage of testing may find success in either topical mucosal
application or intravenous route of administration. These routes of delivery are
chosen because they eliminate or minimize many of the variables of absorption,
distribution, metabolism and elimination. The topical application places the
drug directly on the mucosal membrane. Systemic side effects can be minimized
and local toxic effects can be observed. The therapeutic effect is measured in
the population response as decrease in disease rate of spread.
[0059] Intravenous administration places the drug directly into the blood.
However, toxic effects may be amplified because of this route. To minimize toxic
side effects a slow continuous infusion or a multiple bolus dosing can be used.
The serum drug concentration is monitored to develop a concentration response
curve. The infusion rate or bolus dose and frequency is altered to maintain a
drug concentration or to increase levels. The effect or therapeutic benefit is
measured by periodic measurement of total viral load and p24 concentration. A
common known reversible side effect of polymeric sulfates is an increase in the
APTT or bleeding time. Therefore, in tests involving compounds of the present
invention, the APTT is monitored and maintained at pre-selected values. The
platelet count is also monitored in that thrombocytopenia is a possible expected
reversible side effect.
[0060] Experimental results indicate that the compounds of the present invention
provide unexpected and extended modes of action. Therefore, it is expected that
the antiviral activity of the compounds of the present invention is not limited
to a single viral agent. Target viruses for the evaluation of prior art
antimicrobials include HIV, herpes viruses such as cytomegalovirus and herpes
simplex, hepatitis agents, and the papilloma virus. Efficacy of the compounds of
the present invention in treatment of these species is therefore not unexpected.
[0061] The object of antiviral drug therapy, such as anti-HIV drug therapy, is
to produce and maintain a therapeutic response. The response may be as vague as
a feeling of improvement or the precise measurement of a parameter such as viral
load or serum p24 levels. Attempts have to be made to minimize toxic side
effects while achieving the goal of a therapeutic response. Adjustments in the
dosing form, amount, dosing interval, adjuvant therapy, supportive
chemotherapeutics and expected response window.
[0062] Pharmacokinetic parameters relate the amount of drug in the body or serum
concentration to desired effect rather than relating the dose amount or dose
frequency to the desired effect. However, the practical matter is to first
determine the dose amount and frequency which produces the desired effect and
then to describe this by determining the drug serum concentration. In-vitro
experiments help to describe a rough estimate of concentration of active drug
which produces a specific response. In-vitro experiments also demonstrate, on a
cellular level, toxicity. The ratio of the concentration which produces a
therapeutic response and the concentration which produces a toxic response is
termed the therapeutic index.
[0063] The goal, however, is to determine the therapeutic concentration in a
patient with disease. The goal is to reverse disease. Toxic effects are judged
with regard to the therapeutic benefit. The goal is to place in check toxic
effects so that the drug concentration can be increased and maintained. A
patient population must be studied to overcome the natural variability of
response traditionally observed from patient to patient when treating disease.
The goal of maintaining a therapeutic response can then be achieved.
EXAMPLES
Example 1
Purification of Dextrin
[0064] Type I corn starch dextrin of USP grade having a molecular weight
distribution of approximately 30% of 2,000 to 4,000 daltons and 60% of 8,000 to
10,000 daltons as determined by gel permeation chromatography is supplied. The
dextrin is purified by dissolving into sufficient purified water and dialyzing
against purified water. The dialysis membrane has a pore size of 3000 to 6000
daltons so that smaller size dextrin and impurities are eliminated. The purified
starting material is then dried by lyophilization and is obtained as a white
fluffy solid, melting point 266-274.degree. C. with decomposition.
Example 2
Synthesis of Polysulfate Polymethylsulfate Dextrin
[0065] To 10 mL of dry pyridine is added 1.0 mL of methanesulfonyl chloride and
1.0 mL of chlorosulfonic acid. To this is added 500 mg of dextrin. The mixture
is heated to 55.degree. C. for a period of twelve hours. Ten grams of sodium
hydroxide in 100 mL of water is then added. The aqueous layer is transferred to
a dialysis membrane and dialysed against water until the pH is neutral. The
polysulfate polymethylsulfate dextrin is obtained as a fluffy white solid by
removal of the water by lyophylization. Weight 455 mg; melting point 185-215
degrees Celsius with decomposition 215-220 degrees Celsius. Elemental analysis
shows carbon 31.27%, hydrogen 6.38%, and sulfur 11.28%. The 300 MHZ NMR in
deuterium shows a broad singlet at 5.8 to 5.4 ppm and a broad quartet at 4.5 to
3.2 ppm.
[0066] The methysulfate group may be added to any other sulfates that have been
tested for antiviral activity such as dextrin sulfate, dextran sulfate, cyclo-dextrin
sulfate, or other non-polymeric sulfated structures using this reaction.
Example 3
Synthesis and Purification of Polysulfate Polymethylsulfate Dextrin from
Sulfated Dextrin
[0067] To 10 mL of clean dry pyridine is added 1.0 mL of methanesulfonyl
chloride. The addition requires stirring and cooling. This mixture is then
heated to 55.degree. C. To this is added 500 mg of sulfated dextrin with
stirring. The mixture is heated to 55.degree. C. and stirred for a period of
twelve hours. The mixture is then cooled and ten grams of cooled sodium
hydroxide in 100 mL of water is slowly added with stirring and cooling.
[0068] The aqueous layer is allowed to separate and is transferred to a dialysis
membrane and dialyzed against purified water until the pH of the water remains
neutral. The polysulfate polymethylsulfate dextrin is obtained as a solid by
removal of the water by lyophilization.
[0069] The above synthesis can be applied to any form of sulfated dextrin such
as dextrin-2-sulfate, dextrin-3-sulfate, dextrin-6-sulfate or multiple sulfates.
Any molecular weight of sulfate dextrin can be used such as those with a
molecular weight of 3000 to 10,000 and higher polymers with a molecular weight
of, for example, 10,000 to 500,000.
Example 4
Synthesis of Polysulfate Polymethylsulfate Dextrin with Sulfurtrioxide Pyridine
Complex and Purification Thereof
[0070] (a) Production of the Solid Product: 300 mL of dry pyridine is added to a
reaction flask heated to 20.degree. C. 120 mL of chlorosulfonic acid is slowly
added to the flask, keeping the temperature no higher than 20.degree. C. 120 mL
of methanesulfonyl chloride is added over 15 minutes, keeping the temperature
below 30.degree. C. Another 300 mL pyridine is added to the mixture, and then 95
g of sulfurtrioxide pyridine complex (PySO.sub.3) is added, keeping the
temperature below 40.degree. C. The presence of any solids is determined and
then the mixture is heated to 55-60.degree. C. If a bulk of un-dissolved salts
are present in the mixture, then 50 mL of pyridine is added every 2-3 minutes up
to a maximum of 300 mL of additional pyridine. When the mixture is homogeneous,
152.93 g of dry dextrin is stirred into the mixture and the mixture is heated to
between 55-60.degree. C. for one hour. After one hour, the mixture is cooled and
stirred overnight at room temperature. The final product is a solid. The
pyridine is decanted from the solids and retained. Then the solids then are
removed using a first wash solution, described below. The solids are filtered
using a Buchner funnel and Whatner filter paper # 4. To assist drying of the
solids, a latex sheet can be placed over the solids in the Buchner funnel during
the filtration process. The solid product then is washed with two wash solutions
in the following order: The first wash is made up of ice cold 97.5% acetone and
2.5% HCl (v/v). The volume of this wash should be approximately 500-1000 mL.
This removes most of the pyridine and deactivates the remaining reagent. The
second wash is made up of about 500 mL ice cold 100% acetone. This removes
excess acid.
[0071] (b) Neutralization and Purification of the Solid Product: The solid
product first is made basic by dissolving it in 10% NaOH. The pH of the solution
should be between 10 and 11. The solution then is transferred to a dialysis
membrane for dialysis. The amount of base is determined by the pH reading and
the amount of water is determined by the dialysis step. A large amount of excess
base is not favorable and dialysis limits the amount of water that can be used.
Purification of the product is achieved by dialysis against a 1000 MW cut off
membrane. The dialysis membrane thus has a smaller pore size than the
purification step. Dialysis proceeds with water exchanges until the exchange
water pH is neutral, which takes about 72 hours and requires about 6 water
changes done about every 6-8 hours. After the exchange water has neutralized, it
may be assumed that the product also has a neutral pH. The product then is
removed from the dialysis membrane and placed on a lyophilizer for immediate
freeze-drying. The water is removed by the freeze-drying method so as not to
destroy the product. The polysulfate polymethylsulfate dextrin product is
obtained as a slightly acrid, tan solid by removal of the water by
lyophilization. Weight: 125 g; pH: 7.5; melting point: 185-215.degree. C. with
decomposition at about 215-220.degree. C. Elemental analysis shows carbon:
18.24%; hydrogen: 3.42%; nitrogen: 0.38%; sulfu:r 15.91%; and oxygen: 49.45%.
Percentage organic matter: 67% (ash: 33%).
Example 5
In Vivo Toxicity Study of Polysulfate Polymethylsulfate Dextrin with
Sulfurtrioxide Pyridine Complex in Rats
[0072] (a) Intraperitoneal Administration: Sprague-Dawley rats weighing
approximately 250 g were injected i.p. with increasing amounts of polysulfate
polymethylsulfate dextrin dissolved in sterile water. The LD.sub.50, calculated
by semi-log plot of the data, was 47 mg/kg body weight.
[0073] (b) Oral Administration: Sprague-Dawley rats weighing approximately 250 g
were orally gavaged with increasing amounts of polysulfate polymethylsulfate
dextrin dissolved in sterile water up to a dose of 2 g/kg body weight. No toxic
effects of the compound was observed, thus indicating that oral administration
was "non-toxic."
Example 6
Anti-HIV Testing of Polysulfate Polymethylsulfate Dextrin
[0074] Anti-HIV activity of polysulfate polymethylsulfate dextrin was
demonstrated in cell culture by inhibition of cell-to-cell transmission of the
Human Immunodeficiency Virus as measurement of the p24 protein production in the
presence of increasing drug concentration. The average of three separate tests
demonstrated that the calculated 50% inhibition (IC50) is 1.16 .mu.M. Testing
was performed independently at the NIH using standard testing protocol. Results
are shown in Table 5.
Example 6
Oral Administration of Antiviral Compound for Treatment of HIV
[0075] Oral administration is the most preferred route of administration for
general distribution of the invention allowing ease of dose manufacturing and
dispensing. Absorption through the gut wall is substantial and adequate because
of the increase in lypophilic character of the methylsulfate groups compared to
the sulfate groups alone. The decrease in molecular weight by elimination of the
linear polymer connecting the branch point structure also increases transport
across the gut wall as compared to the limit dextrin. Formulation of the
invention with solubilizing lipid carriers, buffered excipients, and dissolution
enhancers maximizes absorption. The first pass hepatic clearance is expected to
be substantial and should be overcome by increasing the oral dose amount and
dosing frequency.
[0076] Formulation for oral absorption may include any of the following
excipients: glycerin USP, microcrystalline cellulose, methylcellulose, starch,
paraben, methylparaben, colloidal silicon dioxide, magnesium stearate,
simethicone, sorbitol, water, FD&C color, and flavor.
[0077] EXAMPLE FORMULATION: 1 gram of antiviral composition of the present
invention in a soft gel capsule.
[0078] EXAMPLE DOSAGE: 1 capsule four times a day.
[0079] PURPOSE: To determine the effectiveness of the antiviral composition of
the present invention towards the treatment of HIV as the drug is administered
orally.
[0080] METHODOLOGY: The study is an open label study. Subjects are given monthly
supplies of the medication. The subjects self-administer the medication and make
records in a daily journal. The subjects are medically examined monthly, which
may include serum blood drug levels, viral titer or anti-body measurement, serum
chemistry measurements, and serum bleeding parameters.
[0081] Patients take medication at a starting dose which is adjusted on a
monthly basis. If the medication is tolerated and the viral load has not
decreased, then the medication is increased from 10% to 1000%. If the medication
is not tolerated the medication will be decreased 10% to 100%.
[0082] INCLUSION CRITERIA: HIV infection as documented by ELISA or EIA and
confirmed by a Western blot analysis.
[0083] EXCLUSION CRITERIA: Known allergy to the medication.
[0084] END POINT: Elimination of HIV infection.
Example 8
Intravenous Administration of Antiviral Compound for Treatment of HIV
[0085] Intravenous administration is the most preferred route of administration
for initial clinical trials because it ensures that the invention reaches the
systemic circulation. Administration is best accomplished through a large
catheter in the femoral or sub-clavian vein to avoid the complication of small
vein irritation. Dosing protocol is variable to include one time bolus dosing,
multiple dosing protocols which vary the amount of the drug and/or the time
interval between dosing, or continuous infusion.
[0086] Formulation for intravenous administration may contain any of the
following excipients: sterile water, saline, phosphate buffer, dextran, and
sodium hydroxide.
[0087] EXAMPLE FORMULATION: Sterile solution 15 mg/mL "antiviral composition" in
0.9% sodium chloride adjusted to pH 6.0 to 7.5 with 0.01N sodium hydroxide
sterilized with a 0.2 .mu.m filter.
[0088] EXAMPLE DOSAGE: 100 mg of "antiviral composition" per 24 hour period
delivered over a four hour infusion.
[0089] PURPOSE: To determine the effectiveness of the invention "antiviral
composition" towards the treatment of HIV as the drug is administered
intravenously.
[0090] METHODOLOGY: The study is an open label study. Subjects are given daily
doses of the medication. The medication is given in a medical setting and
records in a daily chart are kept. The subjects are medically assessed daily, as
need be, which may include serum blood drug levels, viral titer or anti-body
measurement, serum chemistry measurements, and serum bleeding parameters.
[0091] Patients are administered medication at a starting dose which is adjusted
on a daily basis. If the medication is tolerated and the viral load has not
decreased then the medication is increased from 10% to 1000%. If the medication
is not tolerated the medication is decreased 10% to 100%.
[0092] INCLUSION CRITERIA: HIV infection as documented by ELISA or EIA and
confirmed by a Western blot analysis.
[0093] EXCLUSION CRITERIA: Known allergy to the medication.
[0094] END POINT: Elimination of HIV infection.
Example 9
Intraperitoneal Administration of Antiviral Composition for the Treatment of HIV
[0095] Intraperitoneal administration is the least preferred route of
administration used for general use or for initial clinical trials. The benefit
of intraperitoneal administration is the possible reduction of systemic toxic
side-effects: circulating white blood cells are exposed to the drug invention.
The drug invention is formulated in a phosphate buffer, a pH adjusted saline
solution, a dextrin solution, a lipid emulsion or a combination.
[0096] Formulation for intraperitoneal administration may contain any of the
following excipients: sterile water, saline, dextrin, icodextrin, phosphate
buffer.
[0097] EXAMPLE FORMULATION: 0.015% w/v of "antiviral composition" in 4%
icodextrin solution.
[0098] EXAMPLE DOSAGE: 100 mg of "antiviral composition" per 24 hour period
delivered the intraperitoneal cavity.
[0099] PURPOSE: To determine the effectiveness of the invention "antiviral
composition" towards the treatment of HIV as the drug is administered
intraperitoneally.
[0100] METHODOLOGY: The study is an open label study. Subjects are given daily
doses of the medication. The medication is given in a medical setting and
records in a daily chart are kept. The subjects are medically assessed daily, as
need be, which may include serum blood drug levels, viral titer or anti-body
measurement, serum chemistry measurements, and serum bleeding parameters.
[0101] Patients are administered medication at a starting dose which is adjusted
on a daily basis. If the medication is tolerated and the viral load has not
decreased then the medication is increased from 10% to 1000%. If the medication
is not tolerated the medication is decreased 10% to 100%.
[0102] INCLUSION CRITERIA: HIV infection as documented by ELISA or EIA and
confirmed by a Western blot analysis.
[0103] EXCLUSION CRITERIA: Known allergy to the medication.
[0104] END POINT: Elimination of HIV infection.
Example 9
Topical Administration of Antiviral Composition for Prevention of HIV
[0105] Topical administration is a possible preferred route of administration
for initial clinical trials because it may eliminate systemic absorption
difficulties and toxicities. Administration is controlled by the subject; the
formulation is self-administered. Dosing protocol is variable to include one
time bolus dosing as well as multiple dosing protocols which vary the amount of
the drug and/or the time interval between dosing.
[0106] Formulation for topical administration may contain any of the following
excipients: petroleum jelly, petroleum ointment mixture, sterile water, saline,
phosphate buffer, and dextran.
[0107] EXAMPLE FORMULATION: 0.1% ointment; petroleum based ointment with a pH
buffer of 6.8.
[0108] EXAMPLE DOSAGE: 0.5 gram of ointment within one hour before and one hour
after intercourse to vaginal mucosa.
[0109] PURPOSE: To determine the effectiveness of the invention "antiviral
composition" towards the prevention of HIV as the drug is administered
topically.
[0110] METHODOLOGY: The study is an open label study. The study population
contains 1000 females who are sexually active with a high risk male population.
A known population transmission rate or an untreated group may act as controls.
Subjects are given a supply of individual doses of the medication. The
medication is self-administered. The subjects are medically assessed weekly, as
need be, which may include physical and pelvic examination, serum blood drug
levels, viral titer or anti-body measurement, serum chemistry measurements, and
serum bleeding parameters.
[0111] Patients are administered medication at a starting dose which is adjusted
on a daily basis. If the medication is tolerated and the viral load has not
decreased then the medication is increased from 10% to 1000%. If the medication
is not tolerated the medication is decreased 10% to 100%.
[0112] INCLUSION CRITERIA: Free of HIV infection as documented by ELISA or EIA.
[0113] EXCLUSION CRITERIA: Presence of HIV infection and known allergy to the
medication.
[0114] END POINT: Presence of acquired HIV infection.
[0115] The above invention has been described with reference to the preferred
embodiment. Other modifications and alterations will occur to others upon
reading and understanding the preceding detailed description. It is intended
that the invention be construed as including all such modifications and
alterations insofar as they come within the scope of the appended claims or the
equivalents thereof.
Medical information: Global Humanceuticals, Inc. does not intend to provide specific medical advice or treatment. Global Humanceuticals, Inc. intends to provide the website visitors with documents and information to better understand HIV / AIDS and its prevention and treatment.