 |
Description  |
|
|
BACKGROUND OF THE INVENTION
This invention relates to a process for the production of stable,
lyophilized erythrocyte preparations sensitized by coating with an antigen
or antigen-protein conjugate, respectively which are useful for the
quantitative determination of the antigen, e.g., in hemagglutination
reactions. More particularly, the process of this invention is
characterized by combining erythrocytes, antigen, glutaraldehyde and
formaldehyde in the presence of a buffer solution, allowing the components
to simultaneously act on each other under continuous agitation, washing
and subsequently lyophilizing the thus-coated erythrocytes. This invention
furthermore relates to the erythrocyte preparation obtained according to
this process.
Red blood cells or erythrocytes (generally from sheep) are widely used in
immunochemical diagnostic techniques, particularly sensitized erythrocytes
to which an immunologically or biochemically active group has been
directly or indirectly bonded for hemagglutination testing. In virtually
all diagnostic procedures employing sensitized erythrocytes, the freshness
of the erythrocytes themselves as well as of the sensitized preparation
has been a key factor necessary to obtain accurate and reproducible test
results. While the preparation of sensitized erythrocyte complexes
requires materials, time and skills not always available in clinical
laboratories, the instability of such preparations has severely limited
commercial exploitation of the potential broad use for such materials
manufactured on a large scale.
The problems encountered in freezing red blood cells are compounded when
using sensitized erythrocytes. Not only must cell wall rupture be
minimized to the greatest extent possible, but this must be done without
adversely affecting the sensitization coating as well.
Suitable antigens known to be useful in sensitizing erythrocytes include
but are not limited to the proteohormones, e.g., corpus luteam hormone
(LH, luteinizing hormone), follicle-stimulating hormone (FSH), growth
hormone (STH, somatotropic hormone), prolactin, insulin, etc., and in
particular human chorionic gonadotrophin (HCG) and human placenta lactogen
(HPL). As these latter two proteohormones in particular are found in the
blood and urine of pregnant women, the quantitative determination thereof
is of great importance in the detection and monitoring of a pregnancy. L.
Wide and C. A. Gemzell developed pregnancy reactions with antigen-bound
erythrocytes and antiserum described in Acta Endocrinol. 35: 261 (1960).
These reactions are useful both for monitoring pregnancies and for the
early determination of pathological manifestations.
Enzymes are also suitable as antigens for sensitizing erythrocytes, e.g.,
glutamate-oxalacetate transaminase (GOT), glutamic pyruvic transaminase
(GPT), lactate dehydrogenase, etc.
Useful antigens also include a great variety of different substances, the
detection of which in the blood, urine or other body fluids by techniques
employing sensitized erythrocytes is of clinical interest. Among these
substances are peptide hormones, e.g., oxytocin and angiotensin; steroid
hormones, e.g., testosterone, estradiol, hydrocortisone, etc.; medicinal
agents and drugs, e.g., fluocortolone, lysergic acid diethylamide, etc.
It will be readily apparent that rapid quantitative determinations of all
these substances for diagnostic purposes and for control or screening
examinations are of great value to clinicians.
Substances having a low molecular weight can be bound to the erythrocytes
directly, if they possess functional groups suitable for cross-linking,
e.g., amino groups, or after the introduction of such groups, for use in
the process of this invention. Since this binding process often causes
damage to the erythrocytes, they can advantageously be first linked with a
high-molecular weight "carrier" protein, which serves to protect the
substance of interest from causing excessive damage to the erythrocytes
during coupling. The linking process resides in the formation of a
chemical bond between the antigen and the carrier protein to form an
antigen-protein conjugate, which is then coupled to the erythrocytes.
Suitable carrier proteins are known and include but are not limited to
albumins of various sources, e.g., bovine serum albumin and rabbit serum
albumin; globulins of various species, e.g., bovine-.alpha.-globulin (BGG)
and equine-.alpha.-globulin; synthetic polypeptides, e.g.,
poly-DL-Ala-poly-(Glu, Try)-poly-Lys and
poly-(Glu,Tyr)-poly-DL-Ala-poly-Lys; etc.
Detection reactions with antigen-coated erythrocytes, or erythrocytes
coated with antigen-protein conjugate, and antiserum are effected, e.g.,
by direct or indirect hemagglutination reactions analogously to the
pregnancy determining and monitoring reactions, described above, as is
known to those skilled in the art e.g., by direct and indirect
hemagglutination (HA), hemagglutination inhibition (HAI), etc.
Antigen-coated erythrocytes have been described, e.g., see L. Wide, C. A.
Gemzell, Acta Endocrinol. 35(1960) 261. However, the coated erythrocytes
are unstable. Several attempts have been made to overcome this
disadvantage by the use of coupling and stabilizing agents in the
production of the erythrocyte preparations.
Thus, many bivalent reagents have been proposed as coupling agents between
antigens and erythrocytes, e.g., bis-diazotized benzidines described in
Int. Arch. Allergy 13:1 (1958); 1,3-difluoro-4,6-dinitrobenzene described
in Immunology 4:49 (1961); toluene-2,4-diisocyanates described in
Immunochemistry 1:43 (1964); 1-ethyl-3-(3-dimethylaminopropyl)carbodiimide
described in J. Immunol. 97:791 (1966); glutaraldehyde described in Brit.
J. Haemat. 7:299 (1961); etc. Since even the coupling-coated erythrocytes
are still readily susceptible to decomposition, the erythrocytes have
further been hardened by treating with formaldehyde prior to coating,
e.g., using the procedure described in Proc. Soc. Exp. Biol. (N.Y.) 99:452
(1958). The processes are thereby made complicated and expensive and, due
to the numerous stages employed, do not always yield reproducible results.
In DOS (German Unexamined Laid-Open Application) 2,132,499, a
serum-diagnostic composition of chorionic gonodotrophin bound to red blood
cells by means of glutaraldehyde as the coupling agent is described. In
order to increase the stability of the sensitized erythrocytes, these
blood cells are aftertreated with glutaraldehyde or formaldehyde. The
sensitized blood cells are obtained in the form of a suspension in a
buffer solution. The aftertreatment with glutaraldehyde or formaldehyde
renders the process expensive; furthermore, the HCG-sensitized red blood
cells can be satisfactorily preserved in the suspension only if the latter
is stored under refrigeration at 2.degree.-8.degree. C.
OBJECTS OF THE INVENTION
Accordingly, it is a general object of this invention to provide an
economical process for preparing sensitized erythrocytes useful in
immunochemical techniques.
Another object of this invention is to provide a process for preparing
sensitized erythrocyte preparations having improved stability and extended
shelf life.
A further object of this invention is to provide sensitized erythrocyte
preparations which are stable at room temperature.
An additional object of this invention is to provide a process for
preparing sensitized erythrocyte preparations having improved consistency
of activity from batch to batch.
Upon further study of the specification and appended claims, further
objects and advantages of this invention will become apparent to those
skilled in the art.
SUMMARY OF THE INVENTION
Briefly, the above and other objects are attained in one aspect of the
present invention by providing a process for the preparation of
hemagglutination sensitized, antigen-coated erythrocytes suitable for use
in immunochemical diagnostic techniques, which comprises:
a. admixing a suspension of washed erythrocytes in an aqueous solution
containing an erythrocyte-coupling amount of glutaraldehyde, a
coupled-glutaraldehyde-complexing amount of an erythrocyte-sensitizing
antigen or antigen-protein conjugate and an erythrocyte-hardening amount
of formaldehyde, under incubation conditions at a pH of 5.5 - 8.5 for a
period of time sufficient to form erythrocytes sensitized to
hemagglutination by the coupling of said antigen or antigen-protein
conjugate thereto; and
b. recovering said sensitized erythrocytes from said admixture.
DETAILED DISCUSSION
It has now been found that a stable, lyophilizable antigen or
antigen-protein-conjugate-coated erythrocyte preparation can be obtained
by allowing the erythrocytes, the antigen, glutaraldehyde and formaldehyde
to interact simultaneously on one another in a buffer solution. After the
thus-coated erythrocytes have been washed, the preparation can be obtained
in the solid form by lyophilizing. The lyophilized erythrocyte preparation
is stable at room temperature. The process can be conducted in a single
reaction vessel and can be utilized with a wide variety of different
antigens and/or antigen-protein conjugates.
In accordance with a preferred embodiment, the erythrocytes are coated in
an aqueous solution maintained at a pH of 5.5 to 8.5, preferably of about
7.0 to 7.2. Suitable buffers can be used; these are well known in the art
and include but are not limited to phosphate buffers, borate buffers, tris
buffers, etc. The required buffer strength must be sufficient to maintain
the pH in the range of 5.5 to 8.5 throughout the reaction.
Suitable concentrations of the various reactants, in vol. %, are
approximately:
______________________________________
USEFUL PREFERRED
______________________________________
4 - 12 % 6 - 10 % erythrocytes
0.2 - 2 % 0.4 - 1 % glutaraldehyde
0.6 - 6 % 1 - 4 % formaldehyde
0.01-0.25 %
0.02-0.125% antigen or antigen-
protein conjugate (wt./
vol., as protein)
isotonic 0.08-0.3 mNaCl
ionic strength
______________________________________
The required reaction time depends on the stable incubation or reaction
temperature employed, which can be varied from the freezing point of the
admixture or its components to the denaturation temperature of the protein
or erythrocytes therein. Incubation periods of about 1 and 12 hours and
temperatures of about 5.degree.-45.degree. C are generally required. At
the preferred incubation temperature of about 37.degree. C, the reaction
is usually terminated after about 4 hours.
The coated erythrocytes are washed in the buffer solution until free of
unreacted material, and can then be suspended for freeze-drying in a fresh
buffer solution having a pH of 5-8, preferably 6.2 - 6.5. It is
advantageous to provide that the second buffer solution additionally
contains 0.005 - 0.2 % gelatin, 0.1 - 2 % glycine, and 0.05 - 0.5 %
polyvinylpyrrolidone, e.g., BASF "Kollidon". The latter and gelatin effect
an improved re-suspendability of the erythrocytes, while glycine protects
the preparation from damage during freeze-drying. The freeze-dried
preparation can be conveniently stored, e.g., in hermetically sealed
ampoules under a nitrogen atmosphere.
Without further elaboration, it is believed that one skilled in the art
can, using the preceding description, utilize the present invention to its
fullest extent. The following preferred specific embodiments are,
therefore, to be construed as merely illustrative and not limitative of
the remainder of the disclosure in any way whatsoever. In the following
Examples, the temperatures are set forth uncorrected in degrees Celsius;
unless otherwise specified, all parts and percentages are weight per
volume.
EXAMPLE 1
Production of an HPL-Coated Lyophilized, Stable Erythrocyte Preparation
Starting Materials:
1. Sheep erythrocytes (obtained from Behringwerke, Marburg, West Germany)
2. HPL, human placenta lactogen (95% pure, from Nutritional Biochemicals
Corp., Ohio)
3. Aqueous glutaraldehyde solution, 25% (g/g)
4. Aqueous formaldehyde solution, 35% (g/g)
5. Phosphate buffer I, consisting of 0.075 m NaH.sub.2 PO.sub.4 + 0.45%
NaCl, pH 7.2, 0.01% thimerosal ("Merthiolate")
6. Phosphate buffer II, consisting of 0.019 m NaH.sub.2 PO.sub.4 + 0.11%
NaCl, pH 6.4, 0.31% pulverized gelatin, 0.56% glycine (pro analysis),
0.125% polyvinylpyrrolidone ("Kollidon 25") and 0.0025% thimerosal
("Merthiolate")
Pretreatment:
The sheep erythrocytes are washed twice with a two-fold volume of
physiological saline solution and once with phosphate buffer I. The
washing liquid is separated after each wash by centrifuging the suspension
at 750 g.'s in a refrigerated centrifuge at 4.degree. C. After washing,
the erythrocytes are brought to an 8% suspension in phosphate buffer I.
The percentages for the erythrocyte suspensions refer to hematocrit values
determined after centrifuging at 100 g.'s for 10 minutes.
Treatment:
To 1 part by volume of the washed 8% erythrocyte suspension in phosphate
buffer I are added 0.5 part by volume of a 0.66% glutaraldehyde solution
in phosphate buffer I, 0.5 part by volume of a 2% formaldehyde solution in
phosphate buffer I, and 1 part by volume of a 0.05% HPL solution in
phosphate buffer I.
The resultant admixture is incubated for 4 hours at 37.degree. C in an
obliquely positioned round vessel which rotates slowly about its own axis.
The incubated erythrocytes are then washed three times in phosphate buffer
I, and separated at 250 g.'s in the cooled centrifuge.
The thus-coated erythrocytes are re-suspended in phosphate buffer II as a
0.75% suspension, dispersed in 2 ml aliquots into ampoules, frozen by
immersion of the ampoules into a mixture of methanol and dry ice, and
freeze-dried under dry nitrogen at a pressure of 0.01-0.1 mm. Hg.
absolute. The freeze-dried erythrocytes are subjected to a post drying
step for about 24 hours in a desiccator over P.sub.2 O.sub.5 before the
glass ampoules are sealed by melting. The freeze-dryer and the desiccator
are both purged and maintained under an atmosphere of dry nitrogen, which
is also used to replenish the vacuum following lyophilization.
The freeze-dried erythrocyte preparation produced in this manner exhibits
about 95-100% of the activity of the fresh preparation immediately after
lyophilization (as determined by hemagglutination) and is stable at room
temperature for 6 - 12 months and at 37.degree. C for 1 - 3 months.
EXAMPLE 2
Production of an HCG-Coated Lyophilized, Stable Erythrocyte Preparation
Following the protocol of Example 1, but with the use of HCG, human
chorionic gonadotrophin (5000 IU/mg.) in place of HPL, analogous results
are obtained. The lyophilized preparation has 95-100% of the activity of
the freshly prepared complex (as determined by hemagglutination), and is
stable at room temperature for 6 - 12 months and at 37.degree. C for 1 - 3
months.
EXAMPLE 3
Production of a DNP.sub.3 -BGG-Coated Lyophilized, Stable Erythrocyte
Preparation
Following the protocol of Example 1, but with the use of DNP.sub.3 -BGG
(dinitrophenyl-bovine-.gamma.-globulin) in place of HPL, analogous results
are obtained. The lyophilized preparation has 95-100% of the activity of
the freshly prepared complex (as determined by hemagglutination), and is
stable at room temperature for 6 - 12 months and at 37.degree. C for 1 - 3
months.
EXAMPLE 4
Production of a Fluocortolone.sub.40 -BGG-Coated Lyophilized, Stable
Erythrocyte Preparation
Following the protocol of Example 1, but with the use of fluocortolone-BGG,
fluocortolone.sub.40 -bovine-.gamma.-globulin, in place of HPL, analogous
results are obtained. The lyophilized preparation has 95-100% of the
activity of the freshly prepared complex (as determined by
hemagglutination), and is stable at room temperature for 6 - 12 months and
at 37.degree. C for 1 - 3 months.
The preceding examples can be repeated with similar success by substituting
the generically or specifically described reactants and/or operating
conditions of this invention for those used in the preceding examples.
From the foregoing description, one skilled in the art can easily ascertain
the essential characteristics of this invention, and without departing
from the spirit and scope thereof, can make various changes and
modifications of the invention to adapt it to various usages and
conditions.
* * * * *
|
|
 |
|
 |
Description |
|
