I. FIELD OF THE INVENTION
[0001] The present invention pertains to multi-dose formulations of erythropoietin (hereinafter
"EPO"), comprising a particularly advantageous preservative or combination of preservatives.
Speçifically, the present invention pertains to the use of the preservatives benzethonium
chloride, phenoxyethanol and phenylethyl alcohol, alone or in combination, in multi-dose
EPO formulations. The present invention further relates to a vial for containing a
composition; and a method of inhibiting microbial growth in a solution; wherein all
compositions or solutions comprise EPO and one or more of the preservatives benzethonium
chloride, phenoxyethanol and phenylethyl alcohol.
II. BACKGROUND OF THE INVENTION
[0002] Sterility is one of the most important characteristics of parenteral products. For
parenteral products that are sterilized and intended for single dose injection, maintenance
of sterility is a function of both the method of sterilization and the integrity of
the packaging system. For parenteral products that are intended for multiple dosing,
antimicrobial agents must be added to the product formulation to protect the product
from accidental microbial contamination during its storage and/or use.
[0003] Stable protein-containing multi-dose pharmaceutical formulations are viewed by the
pharmaceutical industry as particularly advantageous and commercially attractive.
Multi-dose formulations are generally, though not always, contained in vials (multi-dose
containers) that allow for the extraction of partial amounts of the formulation at
various times. This type of system is desirable as it allows multiple doses to be
obtained from a single container, and allows for more controlled administration of
the pharmaceutical composition as the formulation may be withdrawn and administered
in any partial amount.
[0004] The nature of the use of multi-dose formulations imposes special requirements on
the formulation. For example, maintenance of the sterility of the composition is particularly
challenging given the many opportunities for introduction of microorganisms and other
contaminants into the formulations. Repeated introduction of foreign elements, for
example, needles, into the multi-dose container after formulation creates a likelihood
of introducing microorganisms into the container. Additionally and alternatively,
microorganisms may be introduced during filling of the containers, or during reconstitution
of the formulations after lyophilization and prior to administration. The extended
periods of time over which the container may be stored - especially during multiple
introductions of foreign elements, and/or after contaminants may have been introduced,
demands that the formulation contain special additives to insure the sterility of
the contents.
[0005] To insure that multi-dose formulations maintain optimally sterile properties, the
United States Food and Drug Administration (FDA) and regulatory agencies in other
jurisdictions require that all multi-dose formulations contain preservatives to prevent
the growth of, or to affirmatively kill, any microorganisms that may be introduced
into the formulations. Given the inherent instability of proteins, and their tendency
to interact adversely with preservative compounds, the development of protein containing
multi-dose formulations has proven particularly difficult. Possible adverse interactions
between preservatives and proteins include the degradation of the protein, especially
when stored for extended periods of time; inactivation of the protein; formation of
protein aggregates; and other interactions that inactivate the formulation or make
administration of the formulation to humans, particularly by infusion, injection or
other parenteral administration, difficult, painful or otherwise undesirable.
[0006] Additionally, preservatives themselves are noted for causing acute adverse reactions,
such as allergic reactions, in humans upon parenteral administration. Ideally, the
preservative contained in the multi-dose protein pharmaceutical composition should
be effective in low concentration against a wide variety of micro organisms, soluble
in the formulation, non-toxic, compatible and non-reactive with the protein, active
with long term stability, and non-reactive with components of the container or closure
system.
[0007] Sandeep Nema
et al. published lists of various excipients that have been included in the formulation
of injectable products marketed in the USA. The antimicrobial preservatives listed
in this review article are included in Table 1:
TABLE 1
| ANTIMICROBIAL PRESERVATIVES |
| Preservative |
Frequency |
Range |
| Benzalkonium chloride |
1 |
0.02% w/v |
| Benzethonium chloride |
4 |
0.01% |
| Benzyl alcohol |
74 |
0.75-5% |
| Chlorobutanol |
17 |
0.25-0.5% |
| m-cresol |
3 |
0.1-0.3% |
| Myristyl gamma-picolinium chloride |
2 |
0.0195-0.169% |
| Paraben methyl |
50 |
0.05-0.18% |
| Paraben propyl |
40 |
0.01-0.1% |
| Phenol |
48 |
0.2-0.5% |
| 2-Phenoxyethanol |
3 |
0.50% |
| Phenyl mercuric nitrate |
3 |
0.001 % |
| Thimerosal |
46 |
0.003-0.01% |
[0008] EPO is a glycoprotein that functions to stimulate the production of hemoglobin and
erythrocytes in bone marrow. It is produced in the kidney, and is widely used as a
treatment for anemia caused by a variety of conditions, including, for example, renal
failure. The amino acid sequence and general glycosylation patterns of EPO are known
in the art. See, for example, Miyaka
et al. and United States Patent No. 4,703,008. Isolation and Purification of EPO, from
human tissues or fluids, has been described by Miyake
et al.
[0009] The nucleic acid sequence encoding the protein, isolation of this sequence, and production
of the protein by traditional recombination methods are also known in the art. See,
for example, United States Patent No. 4,703,008 to Lin, describing the nucleic acid
sequence encoding EPO; United States Patent No. 4,337,513 to Sugimoto
et al., describing the use of lymphoblastoid cells to produce EPO; and Sherwood
et al., describing production of EPO by a human renal carcinoma cell line. Additionally,
production, isolation and purification of the protein is also achievable by gene-activation,
or homologous recombination, followed by well-known isolation and purification techniques.
[0010] Development of EPO-containing multi-dose formulations has proven particularly difficult
by virtue of the particular instability displayed by EPO, and its tendency to readily
interact with common pharmaceutical ingredients. United States Patent No. 4,806,524.
Attempts to develop multi-dose EPO formulations have tried to circumvent these problems
by maintaining the formulations at a low pH, or by including various amino acid constructs,
two approaches thought to assist in the stabilization of the EPO protein, or by developing
lyophilized forms in which the preservative sublimes from the formulation before administration.
United States Patent No. 5,503,827 (the '827 patent) to Woog.
[0011] Stable, sterile multi-dose EPO-containing pharmaceutical formulations are few. They
include those formulations disclosed in the '827 patent. The '827 reference discloses
and specifically claims chloretone (chlorbutanol, 1,1,1-trichloro-2-methyl-2-propanol),
benzalkonium chloride or benzyl alcohol as preservatives. Woog specifically notes
the particular difficulty of providing a multi-dose EPO formulation in which the allergy
rates are reduced, and promotes the use of the specifically claimed preservatives
as especially advantageous in that regard. This reference further stresses that due
to the tendency ofpreservatives to degrade and proteins to be inactivated when combined,
it is most desirable to minimize contact between the preservative and the protein.
The '827 patent further discloses the use of several amino acid constructs and other
additives thought necessary to stabilize EPO in solution. Finally, The '827 patent
discloses, in a most preferred embodiment that any preservative used in the initial
formulation is sublimed away upon lyophilization of the composition. Then, upon reconstitution,
additional preservative selected from the group disclosed (chloretone) as defined,
benzalkonium chloride and benzyl alcohol, may be introduced, but the injectable, reconstituted
solution should be used within 30 days.
[0012] Another example of an EPO-containing multi-dose formulation is described in United
States Patent No. 5,661,125 (the '125 patent). This patent explicitly acknowledges
and affirms other references stating that EPO "is an instable substance especially
in solution form" and "when combined with known stabilizers, the resulting stability
of the EPO is varied and unpredictable." This reference then goes on to show and claim
the specific use of benzyl alcohol, a paraben and/or a phenol or a combination of
these as a preservative in EPO-containing solutions. Further attesting to the difficulty
of discerning compatible and advantageous preservatives for use in EPO-containing
multi-dose formulations, this reference states:
"...nothing specific can be derived from the use of preservatives with other proteins
that would suggest any particular preserved formulation for erythropoietin. See, e.g., Geigert, J., 'Overview of the Stability and Handling of Recombinant Protein Drugs,'
Journal of Parenteral Science & Technology, Vol. 43(5):220-224 (1989)".
[0013] US 5 503 827 discloses multi-dose pharmaceutical preparations containing human proteins
such as erythropoietin and a preservative.
[0014] EP-A-0 459 795 discloses an oral dosage form of erythopoietin containing a surfactant
such as benzethonium chloride.
[0015] Accordingly, there remains a need for an EPO-containing, preserved, multi-dose pharmaceutical
formulation that: (1) maintains the stability of the protein component and the composition
over an extended shelf life of the product; (2) maintains the sterility of the formulation
and meets the United States, European and Japanese Pharmacopia criteria for preservative
challenge testing; (3) is safe in the concentrations used; and (4) is administrable
- by any parenteral or oral route - in a manner that is effective, and minimizes pain
and the chance of adverse reaction, for example, allergic reaction, in the patient.
III. SUMMARY OF THE INVENTION
[0016] The present invention provides a novel and particularly advantageous multi-dose formulation
containing erythropoietin and the preservatives benzethonium chloride, phenoxyethanol
and phenylethyl alcohol, either alone or in combination.
[0017] The formulations of the present invention may be formulated in a variety of concentrations
in various vial sizes for various administration dosages. For example, the formulations
disclosed in the present invention may comprise 10,000, 20,000, 40,000, or even up
to or greater than 100,000 Unit/ml EPO concentrations. They may further contain any
concentrations in between these exemplary concentrations, such as 5,000, 15,000, 25,000
unit/ml concentrations, and the like. Additionally, the dosages may be formulated
in a ½, 1 or 2 ml vial, or any other size vial or other container preferred by the
formulator. It will be clear to one of skill in the art, that any combination of dosages
and vials may be used, depending upon the needs of the formulator. For example, one
could prepare the presently disclosed formulations as a 10,000 unit/½ ml concentration
in a 1 ml vial, a 40,000 unit/ml dose in a 2 ml vial, or any other combination of
concentration of EPO in any size vial. The compositions may be in the form of an aqueous
solution, a suspension, or may be lyophilized.
[0018] The present invention provides in an alternative embodiment, a pharmaceutical carrier
composition, for use as a carrier of EPO, comprising the preservatives benzethonium
chloride, phenoxyethanol, or phenylethyl alcohol, wherein the preservatives are contained
in the EPO carrier composition alone or in combination. The present invention also
provides a vial for containing multiple doses of EPO, wherein the vial comprises EPO
and an effective amount of one or a combination of the following preservatives: benzethonium
chloride, phenoxyethanol, and phenylethyl alcohol.
[0019] In yet another embodiment, the present invention provides a method of inhibiting
microbial growth in an EPO-containing solution, wherein the method comprises adding
to the EPO-containing solution, one or a combination of the following preservatives:
benzethonium chloride, phenoxyethanol, and phenylethyl alcohol.
[0020] Additional components of the EPO multi-dose formulations of the present invention
include surfactants, buffers, osmolality adjusting agents and antiadsorbants. Particularly
advantageous additives include polysorbate-20, polysorbate-80, sodium phosphate, sodium
chloride and genapol.
[0021] The formulations of the present invention may be in solid, semi-solid, liquid or
fluid form, for example, as tablet, aqueous solution or a suspension, or may be lyophilized
and reconstituted prior to administration to a patient. The formulations may be administered
via any parenteral route, including intravenous, subcutaneous, intramuscular, transdermal,
intra-arterial, intra-peritoneal, or via pulmonary inhalation. They may also be administered
orally.
IV. DETAILED DESCRIPTION OF THE INVENTION
[0022] The present invention provides a significant improvement over the state of the art.
Provided are novel EPO-containing multi-dose pharmaceutical formulations containing
preservatives that individually provide for stable, sterile, easily administered compositions.
Further, and most unexpectedly, the present invention discloses that phenoxyethanol
and benzethonium chloride, when used in combination in an EPO-containing multi-dose
pharmaceutical composition, have positive synergistic effects resulting in a particularly
advantageous composition. Specifically, this combination of preservatives displays
the following characteristics: (1) synergistic antimicrobial effect, allowing for
a lower concentration of preservatives to be used; (2) excellent stability of the
EPO, at varying storage conditions, over extended periods of time; and (3) phenoxyethanol
has a potential for a local anesthetic effect, making the composition particularly
preferable for subcutaneous administration.
[0023] As used herein, the following terms have the following meanings:
[0024] Erythropoietin- a glycoprotein which, when in biologically active and glycosylated form, has the
capacity to induce the formation of hemoglobin and red blood cells in bone marrow.
May be obtained via isolation from human tissues or fluids, by traditional recombination
methods, or by gene activation.
Parenteral- by some means other than the gastrointestinal tract; includes intravenous, subcutaneous,
intramuscular, and intramedullary, intra-arterial, intra-peritoneal and pulmonary
inhalation.
Pharmaceutically acceptable (or pharmacologically acceptable)- refers to molecular entities and compositions that do not produce an adverse, allergic
or other untoward reaction when administered to an animal or a human, as appropriate.
Pharmaceutically acceptable carrier- includes any and all solvents, dispersion media, coatings, antibacterial and antifungal
agents, isotonic and absorption delaying agents and the like, that may be used as
a media for a pharmaceutically acceptable substance.
Unit -a unit of biological activity as determined by exhypoxic polyeythemic mouse bioassay
and compared to World Health Organization standards.
[0025] Any numerical values recited herein include all values from the lower value to the
upper value in increments of one unit provided that there is a separation of at least
2 units between any lower value and any higher value. As an example, if it is stated
that the concentration of a component or a value of a process variable such as, for
example, osmolality, temperature, pressure, time and the like is, for example, from
1 to 90, preferably from 20 to 80, more preferably from 30 to 70, it is intended that
values such as 15 to 85, 22 to 68, 43 to 51, 30 to 32 etc. are expressly enumerated
in this specification. For values which are less than one, one unit is considered
to be 0.0001, 0.001, 0.01 or 0.1 as appropriate. These are only examples of what is
specifically intended and all possible combinations of numerical values between the
lowest value and the highest value enumerated are to be considered to be expressly
stated in this application in a similar manner.
A. Preservatives: Phenoxyethanol and Benzethonium Chloride
[0026] The preservatives contemplated for use according to the present invention are preferably
benzethonium chloride, phenoxyethanol and phenylethyl alcohol, any variants of these
preservatives and their structural analogues. It is specifically contemplated that
any of these preservatives may be used as the sole preservative in the presently disclosed
formulations, or they may advantageously be used in combination with each other. As
shown herein, formulations of the present invention using a combination of phenoxyethanol
and benzethonium chloride prove particularly preferable.
[0027] Benzethonium chloride, phenoxyethanol and phenylethyl alcohol may be used in the
presently disclosed formulations in any effective amount. The total preservative concentration
is preferably between about 0.01% and about 4.0% of the total formulation. Particularly
advantageous concentrations of total preservative are those maintained as low as possible
to achieve the requisite antimocrobial effect, while minimizing the potential for
adverse reactions. Although benzethonium chloride, phenoxyethanol and phenylethyl
alcohol can be used individually as preservatives, doing so requires a greater preservative
concentration than if combinations of the preservatives are used.
[0028] In more preferred embodiments of the present invention, both benzethonium chloride
and phenoxyethanol are used together. Surprisingly, when used together these preservatives
have a synergistic effect on one another. To achieve the equivalent antimicrobial
effect when used alone, the concentrations of benzethonium chloride or phenoxyethanol
must each be greater than the total preservative concentration if they are used in
combination and, in general, at least twice as much of the preservative must be used
if employed alone. Thus for example, if either benzethonium chloride or phenoxyethanol
is used alone, approximately at least twice as much benzethonium chloride or phenoxyethanol
will be required to achieve the same effect as an amount of benzethonium chloride
in combination with phenoxyethanol. Further, even at these higher concentrations of
benzethonium chloride and phenoxyethanol, the individual preservative formulations
may not meet United States, European or Japanese anti-microbial regulatory criteria.
Preferred formulations include benzethonium chloride in concentrations of from about
0.01 to about 0.1% in combination with phenoxyethanol in concentrations of from about
0.01 to about 1.0%. More preferred formulations contain benzethonium chloride in a
concentration of from about 0.01% to about 0.02% and phenoxyethanol in a concentration
of from about 0.25% to about 0.5%.
[0029] In another embodiment, the present invention includes benzethonium chloride in combination
with phenylethyl alcohol. Preferred formulations include benzethonium chloride in
concentrations of from about 0.01 to about 0.1% together with phenylethyl alcohol
in concentrations of from about 0.01 to about 1.0%. More preferred formulations contain
benzethonium chloride in a concentration of from about 0.15 to about 0.25% and phenylethyl
alcohol in a concentration of from about 0.2 to about 0.5%. A most preferred formulation
in which benzethonium chloride and phenylethyl alcohol are used in concert, includes
benzethonium chloride in a concentration of about .02% and phenylethyl alcohol in
a concentration of about 0.25%.
B. Erythropoietin
[0030] The nucleic acid sequence, amino acid sequence, three-dimensional structure, and
typical glycosylation patterns of EPO are known in the art. Isolated and purified
EPO from various sources is also known. Accordingly, one of skill in the art can obtain
EPO for use according to the present invention by isolating and purifying the EPO
from human tissue or fluids, through traditional recombinant techniques, and through
gene activation processes. All of these methods are specifically contemplated to be
within the scope of this patent. Additionally, any other EPO, obtained from any source,
is contemplated for use according to the present invention.
C. Other Active Components
[0031] The optimal formulation according to the present invention may vary according to
factors such as amount of time the formulation will be stored, conditions under which
it will be stored and used, the particular patient population to which it may be administered,
etc. Adjustments to the formulation by adjusting constituents of the formulations
and their relative concentrations, other than the preservatives benzethonium chloride,
phenoxyethanol and phenylethyl alcohol and EPO as described
supra, may be made as needed according to the needs of the formulator, administrator or
patient. Additional constituent elements of the multi-dose EPO formulations of the
present invention may include water, a buffer, a surfactant or antiadsorbant, a wetting
agent, and an osmolality adjusting agent. Formulation characteristics that may be
modified include, for example, the pH and the osmolality, to achieve a formulation
that has a pH and osmolality similar to that of human blood or tissues.
[0032] Buffers are useful in the present invention for, among other purposes, manipulation
of the total pH of the pharmaceutical formulation. A variety of buffers known in the
art may be used in the present formulations, such as various salts of organic or inorganic
acids, bases, or amino acids, and including various forms of citrate, phosphate, tartrate,
succinate, adipate, maleate, lactate, acetate, bicarbonate, or carbonate ions. Particularly
advantageous buffers for use in the present invention include sodium or potassium
buffers, particularly sodium phosphate. In a preferred embodiment, sodium phosphate
is employed in a concentration approximating 20 mM. A particularly effective sodium
phosphate buffering system comprises sodium phosphate monobasic monohydrate and sodium
phosphate dibasic heptahydrate. When this combination of monobasic and dibasic sodium
phosphate is used, advantageous concentrations of each are about 0.5 to about 1.5
mg/ml monobasic and about 2.0 to about 4.0 mg/ml dibasic, with preferred concentrations
of about 0.9 mg/ml monobasic and about 3.4 mg/ml dibasic phosphate. The pH of the
formulation changes according to the amount of buffer used. It is preferred to achieve
a pH level of between 5.0 and 8.0, more preferable to have a pH of about 6.0 to about
7.5, and most preferable to develop a formulation with a pH of about 7.0.
[0033] It may also be advantageous to employ surfactants in the presently disclosed formulations.
Surfactants or anti-adsorbants that prove useful according to the present invention
include polyoxyethylenesorbitans, polyoxyethylenesorbitan monolaurate, polysorbate-20,
such as Tween-20™, polysorbate-80, hydroxycellulose, and genapol. In a preferred embodiment,
polysorbate-20 is used. When any surfactant is employed in the present invention,
it is advantageous to use it in a concentration of about 0.01 to abut 0.5 mg/ml. In
a particularly useful embodiment, polysorbate-20 is used in a concentration of about
0.1 mg/ml.
[0034] Additional useful additives are readily determined by those of skill in the art,
according to particular needs or intended uses of the disclosed multi-dose EPO formulations.
One such particularly useful additional substance is sodium chloride, which is useful
for adjusting the osmolality of the formulations to achieve the desired resulting
osmolality. Particularly preferred osmolalities are in the range of about 270 to about
330 mOsm/kg. The optimal osmolality of the presently disclosed formulations is approximately
300 mOsm/kg. ·Sodium chloride in concentrations of about 6.5 to about 7.5 mg/ml are
affective for achieving this osmolality, with a sodium chloride concentration of about
7.0 mg/ml being particularly effective. Or the amount of sodium chloride can be added
or adjusted to achieve an osmolality of about 270 to about 330 mOsm/kg, and preferably
300 mOsm/kg. Other useful osmolality adjusting agents include mannitol and sorbitol.
D. Preparation of the Compositions
[0035] The EPO formulations described herein may be prepared in water suitably mixed with
a surfactant, such as hydroxypropylcellulose or polyoxyethylenesorbitans. In many
cases, it will be preferable to include isotonic agents, for example, sugars or sodium
chloride as described above. Prolonged absorption of the injectable compositions can
be brought about by the use in the compositions of agents delaying absorption, for
example, aluminum monostearate or gelatin. Other agents that may be employed include,
but are not limited to lecithin, urea, ethylene oxide, propylene oxide, hydroxypropylcellulose,
methylcellulose, or polyethylene glycol.
[0036] Aqueous compositions (inocula) as described herein may include an effective amount
of EPO dissolved or dispersed in a pharmaceutically acceptable aqueous medium. Such
compositions are also referred to as inocula. The use of pharmaceutically acceptable
carrier media and agents for pharmaceutically active substances is well known in the
art. Except insofar as any conventional media or agent is incompatible with the active
ingredient, its use in the therapeutic compositions is contemplated. Supplementary
active ingredients also can be incorporated into the compositions as described above.
[0037] A proteoglycan such as EPO may be formulated into a composition in a neutral or salt
form. Pharmaceutically acceptable salts include the acid addition salts (formed with
the free amino groups of the protein) and those that are formed with inorganic acids
such as, for example, hydrochloric or phosphoric acids, or such organic acids as acetic,
oxalic, tartaric, mandelic, and the like. Salts formed with the free carboxyl groups
can also be derived from inorganic bases such as, for example, sodium, potassium,
ammonium, calcium, or ferric hydroxides, and such organic bases as isopropylamine,
trimethylamine, histidine, procaine and the like.
[0038] The therapeutic compositions of the present invention are advantageously administered
in the form of injectable compositions either as liquid solutions or suspensions;
solid forms suitable for solution in, or suspension in, liquid prior to injection
may also be prepared. A typical composition for such purposes comprises a pharmaceutically
acceptable carrier. For instance, the composition may contain 10 mg, 25 mg, 50 mg
or up to about 100 mg of human serum albumin per milliliter of phosphate buffered
saline
[0039] The formulations as described herein may be contained in a vial, bottle, tube, syringe
or other container for single or multiple administrations. Such containers may be
made of glass or a polymer material such as polypropylene, polyethylene, or polyvinylchloride,
for example. Preferred containers may include a seal, or other closure system, such
as a rubber stopper that may be penetrated by a needle in order to withdraw a single
dose and then re-seal upon removal of the needle. All such containers for injectable
liquids, lyophilized formulations, reconstituted lyophilized formulations or reconstitutable
powders for injection known in the art are contemplated for use in the present disclosed
compositions and methods.
V. EXAMPLES
[0040] The following examples are illustrative only and are not to be construed as intended
to limit the scope of the invention.
A. EXAMPLE 1: PRESERVATIVE SELECTION AND STABILITY TESTING
Materials and Methods:
[0041] Sodium phosphate monobasic monohydrate USP, sodium phosphate dibasic heptahydrate
USP, sodium chloride USP/EP, and polysorbate 20 USP/NF were obtained from J.T. Baker,
a division of Mallinckrodt Baker, Inc., Phillipsburg, NH 08865.
[0042] Benzalkonium chloride USP/NF, 2-phenoxyethanol BP, phenylethyl alcohol USP/NF, thimerosal
USP/NF, phenol crystals USP, benzethonium chloride USP/NF, m-cresol USP, phenyl mercuric
nitrate USP/NF, benzyl alcohol USP, chlorobutanol USP, methylparaben USP/NF, and propylparaben
USP/NF were obtained from Spectrum Quality products INC., Gardena, CA 90248.
[0043] Myristyl gamma-picolinium chloride was obtained from Pharmacia & Upjohn Company,
Kalamazoo, Michigan 49001.
[0044] Multi-dose EPO-containing solutions were formulated as sterile, non-pyrogenic, colorless
aqueous solutions in water for injection at 10,000 units and 20,000 units concentration.
Solutions prepared contained a 20 mM phosphate buffer (sodium phosphate monobasic
monohydrate, and sodium phosphate dibasic heptahydrate), 0.01 % w/v polysorbate 20
as an antiadsorbent, 0.45-0.8% w/v sodium chloride (depending on the preservative
system that was used, the amount of sodium chloride was adjusted to produce an Osmolality
of approximately 300 mOsm/kg), and a preservative system. Solutions prepared had a
pH of approximately 7.0, and an Osmolality of approximately 300 mOsm/kg.
[0045] Solutions were sterilized by filtration through a sterile 0.22-micron Millipore filter.
Solutions were packaged in sterile, clear 2 ml USP type 1 glass vials and stored at
5°C and 25°C for chemical stability testing and in sterile 250 - 500 ml HDPP (high
density polypropylene) bottles for microbial testing.
[0046] Preservatives studied included: benzyl alcohol 1.0% w/v, benzalkonium chloride 0.01
% w/v, 2-phenoxyethanol 0.5% w/v, phenylethyl alcohol 0.5% w/v, thimerosal 0.005%
and 0.01% w/v, phenol crystals 0.4% w/v, benzethonium chloride 0.01 % and 0.02% w/v,
m-cresol 0.4% w/v, phenyl mercuric nitrate 0.002% w/v, methylparaben 0.1 and 0.18%
w/v, and propylparaben 0.03% and 0.035% w/v, and myristyl-gamma-picolinium chloride
0.02% w/v. Also, the following
combinations were studied: (1) benzethonium chloride 0.005% w/v with phenoxyethanol 0.25% w/v;
(2) benzethonium chloride 0.005% and phenoxyethanol 0.5% w/v; (3) benzethonium chloride
0.01% w/v with phenoxyethanol 0.5% w/v; and (4) phenylethyl alcohol 0.25% w/v and
benzethonium chloride 0.02% w/v.
Discussion:
[0047] Methyl paraben, propyl paraben, m-cresol, and phenol produced hazy to cloudy solutions
when added to the EPO formulation (buffered solution). This cloudiness problem was
identified as an incompatibility between the absorbent polysorbate 20, and each of
these preservatives (Handbook of Pharmaceutical Excipients, 1994).
[0048] Although chlorobutanol produced a clear solution when used in the formulation, its
evaluation was stopped because it is not stable at pH >3, its half-life at pH 7.5
is approximately 3 months (Handbook of Pharmaceutical Excipients, 1994).
[0049] In the presence of phenyl mercuric nitrate, a cloudy solution was produced. This
cloudiness was identified as an incompatibility between the osmotic agent sodium chloride,
and phenyl mercuric nitrate (Handbook of Pharmaceutical Excipients, 1994).
[0050] Thimerosal produced a clear solution when used in the EPO formulation. Also, it showed
good preservative efficacy. Additionally, the EPO formulation showed good chemical
stability in the presence of thimerosal. However, since it contains mercury, its use
is likely to be unacceptable by the agencies in Europe, Japan and US.
[0051] Formulations containing benzyl alcohol, benzethonium chloride, phenoxyethanol, phenylethyl
alcohol, benzalkonium chloride, and myristyl-gamma-picolinium chloride produced clear
solutions. Based on the minimum inhibitory concentrations for these preservatives,
safety, and frequency of their use, the following preservatives were selected for
further chemical evaluation of the protein stability and anti-microbial effectiveness
of the EPO formulation: benzyl alcohol, berizethonium chloride, phenoxyethanol, phenylethyl
alcohol, and several benzethonium chloride & phenoxyethanol combinations.
B. EXAMPLE 2: STABILITY OF PROTEIN TESTED
Materials and Methods:
[0052] Prototype batches were made using these selected preservatives and placed on stability
at 5°C and 25°C. Samples were tested by a reverse phase HPLC method. The assay results
(% label claim) of the EPO containing formulations in the presence of these preservatives
are shown in Table 2.
[0053] Label claim was determined by reverse phase HPLC using a Waters Delta-Pak□ C18 column
and gradient elution using an aqueous solution containing 0.05% TFA and acetonitrile
concentration which increases from 23 to 86%. Detection of the EPO protein was monitored
at 210 nm.
TABLE 2
ASSAY RESULTS IN TERMS OF CONCENTRATION
(% LABEL CLAIM) |
| Preservative |
Months |
Strength |
Chemical Assay (%LC)1 |
| |
|
|
5°C |
25°C |
| Benzyl Alcohol |
7M |
10,000 U/ml |
98.6 |
90.0 |
| Benzyl Alcohol |
7M |
20,000 U/ml |
99.7 |
93.7 |
| Benzethonium |
4M |
10,000 U/ml |
99.9 |
88.9 |
| Benzethonium |
4M |
20,000 U/ml |
101.5 |
94.4 |
| Phenoxyethanol |
4M |
10,000 U/ml |
100.5 |
96.9 |
| Phenoxyethanol |
4M |
20,000 U/ml |
102.6 |
97.5 |
| Benzethonium & Phenoxyethanol (0.005% & 0.5%) |
3M |
20,000 U/ml |
98.3 |
97.0 |
| 1 as measured by reverse phase HPLC. |
[0054] As can be seen from table 2, the reverse-phase HPLC data show no loss of concentration
of EPO for all formulas when stored at 5 °C for up to 3-7 months. However, formulas
containing benzyl alcohol or benzethonium chloride alone showed up to 10% loss of
EPO when stored at 25 °C for up to 3-7 months. Formulas containing phenoxyethanol
or phenoxyethanol & benzethonium chloride in combination showed no loss of EPO when
stored at 25 °C for up to 3-4 months. These results show the stabilizing effect of
phenoxyethanol and phenoxyethanol & benzethonium chloride in combination on EPO, this
effect is surprising and unexpected as well as extremely advantageous.
C. EXAMPLE 3: PRESERVATIVE CHALLENGE TEST
[0055] Preservative effectiveness tests are Compendial-guided assays that determine efficacy
for preservative systems in multi-dose pharmaceutical preparations. In such assays,
test formulations are challenged with standardized suspensions of indicator aerobic
bacteria and molds and microorganism survival is monitored over a 28-day period.
[0056] Table 3 shows the results of the United States Pharmacopia (USP) and European Pharmacopia
(EP) preservative challenge testing. All tested formulas passed the USP criteria for
preservative challenge test. Formulas containing 0.01% w/v benzethonium chloride,
0.5% w/v phenoxyethanol, or 0.5% w/v phenylethyl alcohol failed the EP criteria for
preservative challenge test. Formulas containing benzethonium chloride and phenoxyethanol
in different combinations and benzethonium chloride and phenylethyl alcohol in combination
passed both the USP and the EP criteria. Based on the data shown in table 3, it appears
that the antimicrobial activity of benzethonium chloride was surprisingly increased
by the addition of phenoxyethanol, in a synergistic manner.
TABLE 3
| PRESERVATIVE CHALLENGE TESTING |
| Preservative |
Strength |
Preservative Challenge |
| |
|
USP |
EP |
| Benzyl Alcohol |
20,000 U/ml |
passed |
not done |
| (1.0%) |
|
|
|
| |
|
|
|
| Benzethonium |
20,000 U/ml |
|
|
| (0.01%) |
|
passed |
failed |
| (0.02%) |
|
passed |
passed |
| |
|
|
|
| Phenoxyethanol |
20,000 U/ml |
passed |
failed |
| (0.5%) |
|
|
|
| |
|
|
|
| Benzethonium & Phenoxyethanol |
20,000 U/ml |
passed |
passed |
| (0.005 & 0.25%) |
|
|
|
| (0.005 & 0.5%) |
|
|
|
| (0.01 & 0.5%) |
|
|
|
| |
|
|
|
| Phenylethyl Alco. |
20,000 U/ml |
passed |
failed |
| 0.5% |
|
|
|
| |
|
|
|
| Benzethonium & Phenylethyl Alco |
20,000 U/ml |
passed |
passed |
| (0.02% & 0.25%) |
|
|
|
REFERENCES:
[0057]
U. S. Pat. No. 4,377,573 to Sugimoto et al.
U. S. Pat. No. 4,703,008 to Lin.
U. S. Pat. No. 4,806,524 to Kawagachi et al.
U. S. Pat. No. 5,503,827 to Woog et al.
U. S. Pat. No. 5,661,125 to Stricklan et al.
Handbook of Pharmaceutical Excipients, second edition, 1994.
L.A. Trissel, "Handbook on Injectible Drugs." Ed. 8, American Society of Hospital
Pharmacists, Inc. 1994.
Miyaka et al., "Purification of Human Erythropoietin," J. Biol. Chem., 252(15):5558-5564, 1997
Physicians' Desk Reference, ed. 48, 1994.
Physicians' Desk Reference, ed. 50, 1996.
Sandeep Nema, R.J. Washkuhn, and R.J. Brendel, "Excipients and Their Use in Injectable
Products," PDA Journal of Pharmaceutical Sciences & Technology, Vol. 51(4), July-August 1997.
Shewood et al., "Erythropoietin Production by Human Renal Carcinoma Cells in Culture." Endocrinology, Vol. 99(2):504-510, 1976.
Sherwood et al., "Establishment of a Human Erythropoietin-Producing Renal Carcinoma Cell Line."
Clinical Research, 31:323A, 1983.
1. Pharmazeutische Zusammensetzung, umfassend Erythropoietin und eine Menge von Benzethoniumchlorid,
die zum Inhibieren von mikrobiellem Wachstum in der Zusammensetzung wirksam ist.
2. Zusammensetzung nach Anspruch 1, die 0,01 % bis 1,0 % Benzethoniumchlorid umfasst.
3. Zusammensetzung nach Anspruch 1, die 0,01 % bis 0,1 % Benzethoniumchlorid umfasst.
4. Zusammensetzung nach Anspruch 1, die 0,01 % Benzethoniumchlorid umfasst.
5. Zusammensetzung nach Anspruch 1, die 0,02 % Benzethoniumchlorid umfasst.
6. Zusammensetzung nach einem vorangehenden Anspruch, die weiterhin Phenoxyethanol umfasst.
7. Zusammensetzung nach einem der Ansprüche 1 bis 5, die weiterhin Phenylethylalkohol
umfasst.
8. Zusammensetzung nach Anspruch 2, die weiterhin 0,01 bis 1,0 % Phenoxyethanol umfasst.
9. Zusammensetzung nach Anspruch 3, die weiterhin 0,1 bis 0,75 % Phenoxyethanol umfasst.
10. Zusammensetzung nach Anspruch 4, die weiterhin 0,25 % Phenoxyethanol umfasst.
11. Zusammensetzung nach Anspruch 4 oder Anspruch 5, die weiterhin 0,5 % Phenoxyethanol
umfasst.
12. Zusammensetzung nach Anspruch 7, die etwa 0,02 % Benzethoniumchlorid und etwa 0,25
% Phenylethylalkohol umfasst.
13. Zusammensetzung nach einem vorangehenden Anspruch, die weiterhin ein Salz umfasst.
14. Zusammensetzung nach Anspruch 13, worin das Salz Natriumchlorid ist.
15. Zusammensetzung nach einem vorangehenden Anspruch, die weiterhin einen Puffer umfasst.
16. Zusammensetzung nach Anspruch 15, worin der Puffer Natriumphosphat ist.
17. Fläschchen, enthaltend eine Zusammensetzung nach einem der Ansprüche 1 bis 16.
18. Verfahren zum Inhibieren von mikrobiellem Wachstum in einer Erythropoietin umfassenden
Lösung, umfassend Zusetzen von Benzethoniumchlorid und gegebenenfalls anderen Komponenten
zu der Lösung zur Bildung einer Zusammensetzung nach einem der Ansprüche 1 bis 16.
1. Composition pharmaceutique comprenant de l'érythropoiétine et une quantité de chlorure
de benzéthonium efficace pour inhiber la croissance microbienne dans la composition.
2. Composition selon la revendication 1, comprenant de 0,01 à 1,0 % de chlorure de benzéthonium.
3. Composition selon la revendication 1, comprenant de 0,01 à 0,1 % de chlorure de benzéthonium.
4. Composition selon la revendication 1, comprenant 0,01 % de chlorure de benzéthonium.
5. Composition selon la revendication 1, comprenant 0,02 % de chlorure de benzéthonium.
6. Composition selon l'une quelconque des revendications précédentes, comprenant en outre
du phénoxyéthanol.
7. Composition selon l'une quelconque des revendications 1 à 5, comprenant en outre de
l'alcool phényléthylique.
8. Composition selon la revendication 2, comprenant en outre de 0,01 à 1,0 % de phénoxyéthanol.
9. Composition selon la revendication 3, comprenant en outre de 0,1 à 0,75 % de phénoxyéthanol.
10. Composition selon la revendication 4, comprenant en outre 0,25 % de phénoxyéthanol.
11. Composition selon la revendication 4 ou la revendication 5, comprenant en outre 0,5
% de phénoxyéthanol.
12. Composition selon la revendication 7, comprenant environ 0,02 % de chlorure de benzéthonium
et environ 0,25 % d'alcool phényléthylique.
13. Composition selon l'une quelconque des revendications précédente, comprenant en outre
un sel.
14. Composition selon la revendication 13, dans laquelle le sel est le chlorure de sodium.
15. Composition selon l'une quelconque des revendications précédente, comprenant en outre
un tampon.
16. Composition selon la revendication 15, dans laquelle le tampon est le phosphate de
sodium.
17. Fiole contenant une composition selon l'une quelconque des revendications 1 à 16.
18. Procédé d'inhibition de la croissance microbienne dans une solution comprenant de
l'érythropoiétine, comprenant l'addition à la solution de chlorure de benzéthonium
et, éventuellement, d'autres composants pour former une composition selon l'une quelconque
des revendications 1 à 16.