`
`PIIARMACOKINETICS/PIIARMACODYNAMICS
`
`Pharmacokinetics of clindamycin HCl administered intravenously,
`
`intramuscularly and subcutaneously to dogs
`
`E. LAVY*
`
`G. 21er
`
`M. SHEM-Tov:
`
`A. GLICKMAN§ &
`
`A.DEYfi
`
`*Koret School of Veterinary Medicine. The
`Hebrew University of Ierusalem, PO. Box
`12, Rehovot 76100, Israel, iVetgenerics
`Research G. Ziv Ltd, P.O. Box 2473
`Rehovot 76124, Israel, §Ministry of
`Agriculture, Kimron Veterinary Institute,
`P.O. Box 12, Bet—Dayan 50250, Israel, and
`filAvinrl Chemie GmbH. Hannover, Germany.
`Tpassed away November 1997
`
`Lavy, E., Ziv, G., Shem-Tov. M., Glickman, A., Dey, A. Pharmacokinetics of
`clindamycin HCl administered intravenously,
`intramuscularly and subcuta-
`neously to dogs]. vet. Pharmacol. Therap. 22, 2617265.
`
`A buffered aqueous solution of clindamycin Hcl (200 mg/mL) was injected
`intravenously (i.v.) intramuscularly (i.m.) and subcutaneously (s.e.) in a non-
`randomized, partial cross—over trial involving six male and six female dogs.
`Blood samples were collected at conventional, predetermined time periods and
`serum drug concentrations were determined by microbiological assay. Dogs
`were observed clinically for signs of pain, and activity of serum creatine
`phosphokinase (CPK) was monitored after i.m. dosing.
`The i.v. data from five of the dogs best fitted a two-compartment open-system
`pharmacokinetic model whereas a non-compartment model was most suitable
`for analysis of the data from the remaining seven dogs. The mean i.v.
`
`elimination half—life (tt/ZB) and the mean residence time (MRT) were 124 and
`143 min, respectively. The mean volume of distribution at steady state (VSS) was
`0.86 L/kg. Little pain was recorded upon i.m. injection; mean peak serum drug
`concentration (Cum) was 4.4 ug/mL, the elimination half-life (ti/261) was 247
`min and the calculated bioavailability (F) was 115% of the i.v dose. Serum CPK
`activity was elevated to 25—fold the pretreatment level in samples collected 4, 8
`and 12 h after
`i.m.
`injection. Pain was not
`recorded after
`s.e. drug
`administration: the mean Cmax of 20.8 ug/mL was significantly greater than
`the corresponding value for the i.m. route, and F was 310%. The s.e. route
`appears to be superior to the i.m. route in terms of local tolerance and serum
`drug level; a 10 mg/kg SID treatment regimen is suggested for treatment of
`canine infections due to clindamycin sensitive bacteria.
`
`(Paper received 16 December 1998; accepted for publication 1 1 May 1999)
`
`E. Lavy, Koret School of Veterinary Medicine, The Hebrew University, PO. Box 12,
`Rehovot 76100, Israel.
`
`INTRODUCTION
`
`A semisynthetic derivative of lincomycin, clindamycin has been
`shown to be clinically effective and is recommended for treatment
`of staphylococcal and anaerobic infections of skin, soft tissue and
`bone in dogs (Berg et al.. 1984: Greene. 1989: Braden et al.. 1988:
`Braden et al., 1987). Clindamycin is available for parenteral
`administration as the 2-phosphate and hydrochloride. Clindainy—
`cin 2-phosphate is microbiologically inactive, but is hydrolized in-
`vivo to clindamycin (Webber et al., 1980). The phar'rnacokinetics of
`clindamycin phosphate in dogs were studied after single intrave-
`nous l:i.v.) and intramuscular (i.m.) administrations at 11 mg/kg
`clindamycin (Webber et al.. 1980) and after single subcutaneous
`(s.e.)
`injections at 2.75, 5.5, 11 and 21 mg/kg clindamycin
`(Webber et al.. 1980). Based on the pharmacokinetics of the drug,
`s.e. dosage regimen of 11 mg/kg of clindamycin free base as
`clindamycin-2-phosphate/kg body weight every 24 h was
`recommended (Budsberg et al., 1992). The i.m. administration of
`clindamycin-2-phosphate solution (50 mg/mL) induced signs of
`
`this route was not
`therefore.
`pain and other side-effects and,
`recommended (Budsberg et al., 1992). A buffered 20% aqueous
`solution of clindamycin hydrochloride (200 mg/mL) is available
`for pharmacokinetic and clinical testing. The purpose of this study
`was to determine the concentrations of clindamycin in normal
`canine serum after single i.v.,
`i.m. and s.e. administrations of
`clindamycin HCl and compare the derived kinetic variables with
`those obtained earlier
`in dogs
`injected with equal doses of
`clindamycin phosphate (Webber et al.. 1980: Budsberg et al..
`1 9 9 2). Local tolerance and appearance of side-effects following i.m.
`and s.c. administrations were particularly examined.
`
`MATERIALS AND METHODS
`
`Animals
`
`Twelve adult mixed breed dogs, six males and six females (4713 kg
`b.w.) were used in the study. All dogs were housed in the test
`facility for 3 weeks prior to the study. Dogs had free access to
`
`@1999 Blackwell Science Ltd
`
`261
`
`AstraZeneca Exhibit 2121 p. 1
`InnoPharma Licensing LLC v. AstraZeneca AB IPR2017-00900
`
`
`
`262 E. Lavy ct al.
`
`water and commercial dry dog ration before and during the study.
`Inclusion criteria included normal findings on physical examina-
`tion, complete blood count (CBC) serum concentrations of urea
`nitrogen, creatinine, albumin,
`total protein glucose, bilirubin,
`triglycerides, cholesterol, calcium, magnesium, sodium, potas-
`sium, chlorides,inorganic phosphorus and serum activities of
`alkaline phosphataes, alanine aminotransferase, aspartate amino-
`transferase and amylase were determined. Dogs selected for the
`study exhibited normal CBC and blood biochemistry test results.
`
`Experimental design
`
`Intravenous protocol
`jugular vein catheters were placed in each dog; patency of each
`catheter was maintained with heparinized saline. A blood sample
`was taken prior to the beginning of the trial. Each dog was given
`the 20% buffered aqueous clindamycin HCl i.v. at 10 mg/kg.
`Blood samples were obtained at 10, 20, 30, 40, 50, 60, 80, 90,
`120. 180, 240, 360, 480 and 600 min post injection. Blood was
`allowed to clot at 20°C for 2 h and was then centrifuged at
`1000 X g; the serum was collected and stored at —20°C until it
`was assayed.
`
`Intramuscular and subcutaneous protocols
`A 2 week rest period was allowed for all dogs. All indwelling
`jugular venous catheter was placed and maintained as for the i.v.
`protocol, and a baseline blood sample was taken. The injection
`site [4 X 4 cm2 area) on the dorsal aspect of the left and right
`sites were then shaved to remove short hair. Nine dogs received a
`single i.m. injection of the 20% clindamycin HCl at 10 mg/kg in
`the left-side of the neck and the remaining three dogs received a
`single i.m. injection of 375 mL sterile physiological saline in the
`neck. Two weeks later, nine dogs were prepared by procedures
`identical to those used before i.m. drug administration. Six dogs
`received a single s.c. injection of 20% clindamycin HCI at 10 mg/
`kg in the right—side of
`the neck. All dogs were observed
`immediately following i.m. and s.c.
`injections for evidence of
`pain. itching or irritation. The injection sites on both sides of the
`neck were palpated at each blood sampling time and at least two-
`times per day on the following 2 days and any abnormal finding
`such as pain, swelling and discoloration were recorded.
`Blood samples were obtained at 15, 30, 60, 90. 150, 210,
`270. 390, 510, 630, 720 and 1440. min post i.m. injection.
`Blood samples were collected at 30, 45, 60, 90, 120, 180, 240,
`360, 480, 600, 720 and 1440 min post s.c. injection. Blood
`samples were processed as for after i.v. injection.
`
`Clindamycin analysis
`Clindamycin concentrations were measured by microbiological
`well/agar plate diffusion assay as previously described (Bennett et
`al., 1966). The assay organism S.
`lutea ATCC 9341, was
`inoculated into antibiotic Medium No.
`1
`(Difco, Detroit, MI,
`USA) and a 7.0 mm layer seeded medium was added to each Petri
`Plates. Six wells, 8 mm in diameter, were cut into the agar at
`equal distances. A 50.0 uL aliquot of samples (and standard
`clincamycin HCl solution) was alternately added to each well and
`
`the plates were incubated at 3 7°C for 14716 h. The concentra-
`tion of drug in each sample was calculated from zone of inhibition
`diameters using polinomial regression techniques. Sensitivity
`limit of assay method was 0.1 iLg/mL. Standard curves were
`derived using clindamycin HCl [Sigma Chemical Co. St. Louis,
`MO, USA)
`in dog serum. The correlation coefficient of the
`standard curve from 0.10 to 6.0 ug/mL was 0.99 (P< 0.001).
`Samples with concentrations > 6.0 ug/mL were diluted with
`antibiotic-free dog serum to bring clindamycin concentrations
`within the range of the standard curve. The coefficients of
`variation of
`repeatedly assayed samples at concentrations
`ranging between 1 6 ug/mL and 0.1 1.0 ug/mL were 7.5%
`and 12.5%. respectively. Samples were assayed in duplicate and
`data are reported as mean i SD. It was recognized that this assay
`fails to distinguish between clindamycin and its putative active
`metabolites and,
`therefore,
`results were expressed as serum
`clindamycin antimicrobial equivalent activity. Thus the term
`‘clindamycin concentration’ where used throughout this report is
`rather clindamycin antimicrobial equivalent activity.
`
`Serum creatine phosphokinase ( CPK)
`Serum CPK values were determined, using as enzymatic method
`(CK-NAC-active creatine kinase EC2.7.3.2, Randox Laboratories
`Ltd., Crumlin, Northern Ireland), in blood samples collected at 0,
`4, 8, 12, 24, 32, 48 and 72 h after nine dogs were injected i.m.
`with 20% clindamycin HCl solution, three dogs were injected with
`saline, three dogs were injected s.c. with 20% clindamycin HCl
`and three dogs were administered saline s.c. As large differences in
`pretreatment CPK values were found among the dogs examined,
`serum CPK data were converted to percentage by dividing each
`post
`treatment value by the pretreatment value for
`the
`corresponding animal. The post treatment CPK data are presented
`as mean i SD-fold rise from pretreatment (baseline) CPK value.
`
`Data analysis
`Estimates of first-order rate constants and volumes were initially
`obtained by subjecting mean data to analysis. using iterative least
`squares regression analysis
`(Brown 8; Manno, 1978). The
`concentrations vs. time data from each dog were then analysed,
`using a microcomputer program for nonlinear weighted least
`square regression (Bourne, 1986).
`The most appropriate pharmacokinetic model was selected
`on the basis of the lowest weighted sum of squares and the
`lowest Akaike’s information criterion (AIC) value (Yamaoka et
`al., 1978) for data from each dog. The i.v., i.m. and s.c. areas
`under the curves (AUCs) were calculated using trapezoidal
`approximations between time of drug administration and 1440
`min afterwards. Differential calculus methods
`[Edwards 8:
`Penney, 1982) were used to estimate peak serum drug
`concentrations (Calm) and time of Cmax (tmax) after i.m. and
`s.c.
`administrations. Kinetic
`values
`are
`presented
`as
`mean : SD; half lives, however. are presented as harmonic
`
`mean : pseudo-SD [Lam et al. 1985). The paired Student’s
`t—test was used for calculating the significance of the differences
`in the mean kinetic values for the i.m. and s.c. routes: P < 0.05
`
`value was considered significant.
`
`@1999 Blackwell Science Ltd, ]. vet, Pharmacol. Therap. 22, 26172 65
`
`AstraZeneca Exhibit 2121 p. 2
`
`
`
`RESULTS
`
`Clinical signs indicative of slight pain were noticed in four to five
`of the dogs immediately following i.m. injection; the remaining
`dogs did not exhibit any pain reaction. Signs suggesting pain or
`discomfort were not shown by any dog after s.c.
`injection.
`Palpation of the injection site did not elicit any pain reaction.
`Local changes could not be felt at the injection site. Thus. the
`neck side injected with clindamycin 1101 could not be differ-
`entiated from the side injection with sterile saline solution.
`Mean serum clindamycin concentrations after i.v., i.m. and
`s.c. administrations are presented (Table 1). Data are also
`presented graphically as mean log10 serum concentrations vs.
`time plot (Fig. 1). The i.v. data from five of the dogs best fitted a
`two-compartment open system pharmacokinetic whereas a 011e-
`compartment model was most suitable for analysis of data from
`the remaining seven dogs. Thus. the kinetic values Cp". A. and
`tI/w presented (Table 2) represent data from these five dogs: it
`shows a rapid rate of drug distribution from the central to the
`peripheral body compartment. The elimination half-life (LI/113) and
`the mean residence time (MRT) were 124.0 i 57.0 min and
`143.0 i 34.0 min. respectively and the steady state volume of
`distribution
`(VSS) was 0.86 i 0.35 Ii/kg. After
`i.m. drug
`administration. the mean Cmax (4.4 i 0.5 ug/mL) was signifi—
`cantly (P < 0.05) lower than the corresponding value for the s.c.
`administration (20.8 i 6.2 ng/mL).
`The mean absorption time (MAT) of clindamycin HCl solution
`injected s.c. was significantly shorter than after i.m. administra-
`tion. The mean tl/zel i.m. value (427.0 i 209.0 min) was not
`significantly different from the mean tyzel for the s.c. route
`(310.2 i 190.4 min) but these values were significantly longer
`than the mean i.v.
`tI/IB. The mean s.c. AUC was significantly
`larger than the mean i.m. AUC and the resulting calculated
`bioavailability (F) values which were 1.15 and 3.1 for the i.m.
`and s.c. routes, respectively (Table 3).
`Serum CPK activity rose sharply within 8 h after i.m/ injection
`of clindamycin HCl: activity returned to pretreatment level by
`48 h post treatment. A minimal rise in serum CPK activity was
`observed after s.c. clindamycin injection. The i.m. and s.c.
`administration of saline did not affect serum CPK activity.
`
`DISCUSSION
`
`(11.,
`The clinical manifestations of pain described (Budsberg et
`1992) following i.m. administration of 5% solution of clindamycin
`phosphate to dogs were not seen at all after i.m. injection ofmore
`concentrated (20%) buffered aqueous solution of clindamycin HCl.
`We can only speculate on the causes for these differences in local
`tolerance; they could be due to the type of clindamycin salt. the
`presence of buffer or a four-fold smaller volume injected using the
`20% clindamycin HCl solution. The transient rise in serum CPK
`activity observed after i.m. injection of clindamycin HCl to dogs
`(Fig. 2) indicates some degree of muscle tissue damage at the
`injection site (Steinnes et (11.. 1978). However. a similar or even
`higher and more persistent rise has been documented for a long
`
`@1999 Blackwell Science Ltd, J. vet. Pharmacol. Therap. 22. 2617265
`
`Mean serum clindamycin concentration in dogs 263
`
`(ng/mL) after
`Table 1. Mean serum clindamycin concentrations
`intravenous, intramuscular and subcutaneous injection of clindamycin
`HCI to dogs at 10 mg/kg body weight
` Treatment
`
`Time
`(min)
`
`10
`15
`20
`30
`40
`45
`50
`60
`80
`90
`120
`150
`180
`210
`240
`270
`360
`390
`480
`510
`600
`630
`720
`1440
`
`Intravenous
`n=12
`Mean
`SD
`
`Intramuscular
`n=9
`Mean
`
`SD
`
`Subcutaneous
`n=6
`Mean
`SD
`
`2.3
`
`2.2
`2.3
`2.5
`
`1.8
`1.4
`0.6
`1.3
`0.87
`
`0.7
`
`0.45
`
`0.22
`
`0.10
`
`0.11
`
`13.4
`NS
`11.3
`10.2
`8.9
`NS
`7.7
`6.8
`5.75
`5.6
`4.1
`NS
`3.0
`NS
`2.1
`NS
`0.82
`NS
`0.46
`NS
`0.31
`NS
`NS
`NS
`
`NS
`2.6
`NS
`3.6
`NS
`NS
`NS
`4.0
`NS
`4.0
`NS
`3.5
`NS
`3.0
`NS
`2.3
`NS
`1.7
`NS
`1.1
`NS
`0.70
`0.60
`0.30
`
`NS
`NS
`NS
`16.8
`NS
`19.5
`NS
`17.4
`NS
`13.5
`12.6
`NS
`10.7
`NS
`6.9
`NS
`4.6
`NS
`3.3
`NS
`2.7
`NS
`1.7
`0.3
`
`12.8
`
`3.8
`
`6.7
`
`4.1
`4.6
`
`3.2
`
`2.2
`
`1.4
`
`1.8
`
`1.6
`
`1.2
`0.1
`
`0.76
`
`0.90
`
`0.60
`
`0.70
`
`0.50
`
`0.40
`
`0.40
`
`0.40
`
`0.40
`
`0.30
`0.30
`0.10
`
`—t-‘ 5-0-
`+ im
`+ W
`
`
`(pg/mL)
`Concentration
`
`870
`
`1160
`
`1450
`
`O
`
`290
`
`580
`
`Fig. 1. Serum clindamycin concentrations (pg/mL. log 10 scale) after
`intravenous, intramuscular and subcutaneous administration of
`clindamycin HC] to dogs at 10 mg/kg.
`
`list of apprived veterinary injectable products which are very
`commonly used in small and large animal practice without any
`observable pain reactions (Rasmussen. 1980; Svendsen. 1983). A
`better safety evaluation of i.m. clindamycin HCl therapy must wait
`until data from multiple injections are available. The present
`
`AstraZeneca Exhibit 2121 p. 3
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`
`
`264 E. Lavy ct al.
`
`Table 2. Selected pharmacokinetic values for clindamycin HCl adminis—
`tered intravenously to 12 dogs at 10 rug/kg
`
`
` Kenetic value 8: unit Mean SD
`
`
`
`3.71
`18.75
`Cpo. pg/mL
`3.35
`11.06
`A, ng/mL
`3.35
`7.54
`B, itg/mL
`13.30
`11.00
`ti/fl. min
`57.00
`124.00
`ti/ZB. min
`34.00
`143.00
`MRT, min
`0.11
`0.56
`Vt, L/kg
`0.35
`0.86
`VSS, L/kg
`280.00
`1457.00
`AUC, ug/mL.min
`1.10
`6.10
`Clt, mL/min/kg
`
`r2 0.031 0.967
`
`
`A = ordinal intercept of fastest disposition slope minus the intercept of the
`slowest disposition slope; B= ordinal intercept of the slowest disposition
`slope: CpO = initial serum concentration; ti/w = distribution half—life;
`ti/zfi.
`elimination half»life; MRT— mean residence time; VC— volume of the
`central compartment; V55= volume of distribution at steady state;
`AUC: area under the concentration—time cutve from zero to 24 11 post—
`treatment; Cl,=total body clearance;
`r2 =c0rrelation coefficient to the
`line of best fit for a two—compartment open system pharmacokinetic.
`
`Table 3. Selected pharmacokinetic values for clindamycin administered
`intramuscularly and subcutaneously to dogs at 10 mg/kg
` Treatment
`
`Kinetic
`value
`and unit
`
`Cmax‘ ug/mL
`tmaxv min
`MAT, min
`tl/lely min
`MRT, min
`AUC, ug/niL min
`PM
`
`Intramuscular
`n= 9
`
`Mean
`
`SD
`
`4.4
`73.0
`546.0
`427.0
`700.0
`1806.0
`1.15
`
`0.5
`16.0
`226.0
`209.0
`246.0
`346.0
`0.19
`
`Subcutaneous
`n = 6
`
`Mean
`
`SD
`
`20.8
`46.7
`224.5
`3 10.2
`364.2
`5258.0
`3.10
`
`6.2
`20.1
`163.5
`190.4
`147.3
`2161.0
`0.22
`
`time to peak serum
`Cm”, peak maximal serum concentration; Lmax,
`concentration; MAT=mean absorption time, calculated as MRTDOWW
`MRTLV‘; F*=bioavailability, calculated as AUCDOU_LV‘/'AUCLV‘
`
`mam Clandalm.
`
`me~ Saline i.m.
`
`
`
`3821
`
`C?
`
`
`
` 24 FaniaI3581mmflagellumwine{mewwSD}
`
`
`
`15
`
`m
`
`45
`
`60
`
`3’5
`
`Time (is)
`
`Fig. 2. Serum CPK activity in dogs after intramuscular administration of
`clindamycin HCl at 10 mg/kg.
`
`findings clearly indicate that the s.c. route is superior to the i.m.
`route in terms of local tolerance.
`
`Interpretation of data gathered in the course of the present
`study must
`take into consideration the assay method used
`(microbiological). Although a good agreement was shown
`between microbiological and chemical (GC) test results in dog
`serum for clindamycin (Ziv & Shem-Tov, unpublished data), there
`is a slight chance that there are some putative active metabolites.
`The disposition curves after i.v. administration of clindamycin
`HCl was best represented as a two-compartment open model in
`only five of the dogs. The i.v study protocol we used called for
`collecting the first post treatment blood sample at 10 min.
`Because of the rapid distribution rate of the drug in the dog
`[ta/10; of 3.5 i 1.1 min) according to (Budsberg et (11., 1992), we
`probably missed observing the distribution phase. Values for the
`other major kinetic parameters found in the present study were
`also different from the values calculated in dogs injected i.v. with
`clindamycin phosphate (Budsberg et (11.. 1992). Thus, mean ti/ZB,
`MRT and AUC after clindamycin phosphate administration were
`194.6 min. 263.4 min and 2009.5 ug-mL. respectively. Such
`differences in kinetic values, although small, could result from
`the rate of appearance of bioactive antibiotic in the serum after
`i.v. administration of the microbiologically inactive clindamycin
`phosphate, differences in body—weight (clindamycin phosphate
`was injected to dogs weighting 20 to 30 kg), (Budsberg et (11..
`1992) or slightly different methods used for calculating the
`kinetic variable. On the other hand, mean Cit, VC, and VSS for
`clindamycin phosphate were very Close to the corresponding
`values for clindamycin HCl estimated in the present study.
`Regardless of these small differences, the large VSS of clindamycin
`indicates possible wide distribution in the body fluids and tissues.
`Direct measurements of tissue clindamycin concentrations in
`humans (Panzer et 61]., 1972; Dhawan 8: Thadepalli, 1982) and
`cats (Brown at £11., 1990) confirmed these assumptions.
`The kinetic variables calculates from the i.m. serum drug level
`data for clindamycin HCl and clindamycin phosphate were in
`good agreement. The short tmax |’_ 1h) and average bioavailability
`of nearly 100% support rapid and complete absorption of the
`drug from the site of i.m.
`injection, as was remarked earlier
`(Budsberg et (11., 1992). The kinetic profile of the drug in serum of
`all dogs after s.c administration of clindamycin HCl
`is rather
`unique; mean Cmax (20.8 ug/mL) was nearly 4.5 times greater
`than the mean i.m. Cmax. Moreover, mean serum concentrations
`during the first 12 11 post treatment by the s.c. route were two to
`three-fold higher than the concentrations found after i.m. drug
`administration (Fig. 1). After a nearly equivalent dose of the drug
`(11 mg/kg) was injected s.c. to dogs as clindamycin phosphate
`[VVebber et
`(11., 1980) a mean Cmax of 6.1 i 0.3 ug/mL was
`recorded at
`tmax of 40760 min. We found that the terminal
`elimination rate of
`the drug from serum [ta/281) after
`s.c.
`administration of 20% clindamycin HCl solution (310.2 i
`190.4 min) was considerably longer than the reported [Budsberg
`et (11.. 1992) ti/zel of 234.8 i 27.3 min after an equivalent dose
`was given to dogs i.m. as clindamycin phosphate. A tn/zel of 13.9 h
`was calculated (Webber et (11.. 1980) from the semm clindamycin
`data of dogs injected s.c. with clindamycin phosphate.
`
`@1999 Blackwell Science Ltd, ]. vet, Pharmacol. Therap. 22. 26172 65
`
`AstraZeneca Exhibit 2121 p. 4
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`
`
`It appears therefore. that s.c. administration of clindamycin
`HCl allows for rapid, complete drug absorption and, at the same
`time, acts as a depot which limits the rate of drug elimination
`from serum. A entero-hepatic circulation effect was suggested to
`operate in dogs treated orally with clindamycin HCl (Lavy ct al.,
`1999) contributing to the prolongation of tI/Zel to nearly 6 h, and
`for calculated oral bioavailability values exceeding 100%.
`Whatever the pharmacokinetic processes involved.
`it appears
`from the present study that the s.c. route is superior to the i.m. in
`practical terms by permitting a longer treatment interval.
`Earlier studies (Braden et al., 1987; Budsberg et al., 1992)
`attempted to establish i.v. and i.m. dosing recommendations
`using average serum concentrations at steady state with the
`accompanying peak (Cpmax) and through (Cpmax) concentrations
`as means for calculating (Gibaldi, 1982; Riviere, 1988) dosage
`regimens for clindamycin phosphate in dogs. The calculated
`dosage schedule was eventually found to be in agreement with
`the currently recommended oral dosage schedule of 1 1 mg/kg, q
`12 h (Budsberg et al., 1992). We have tried to use a similar
`approach for selecting desirable, potentially antibacterial effec-
`tive, serum drug concentrations in dogs given clindamycin HCl
`by s.c. route. In relating the minimal inhibitory concentration
`(MIC) of clindamycin to its pharmacokinetic properties it has
`been assumed (VVebber et al., 1980; Budsberg et al., 1992;
`Brown et al.. 1990: Riviere. 1988)
`that:
`(a)
`tissue drug
`concentration at least equal to the MIC is maintained through-
`out the entire dose interval; (b) the drug is minimally bound to
`serum protein and serum concentrations are equal to, or even
`slightly lower than, the concentration in major target sites of the
`body (excluding bone):
`(c)
`the kinetic profiles of the drug in
`serum and the target tissue on multiple dosing are very similar;
`and (d)
`the MIC for Staphylococcus aureus/intermedius ranges
`from 0.04 to 0.4 ug/mL and for most anaerobic bacteria, the
`MIC ranges from 0.1 to 3.1 ug/mL but the MIC 90 is in effect
`> 1.6 ug/mL (Greene, 1989; Budsberg et al., 1992; Brown et al.,
`1990). Using the mean serum concentration values, we observed
`that a single s.c. 10 mg/kg SID dosage regimen appears to be
`appropriate for clindamycin HCl tOr the treatment of staphylo-
`coccal soft tissue infections. For anaerobic infections, however,
`this treatment should be given BID. A more intensive course of
`clindamycin therapy is apparently required for the treatment of
`staphylococcal bone infections in the dog (Braden et al., 198 7:
`Braden et al., 1988; Budsberg et al., 1991).
`
`REFERENCES
`
`Bennett, J.V., Brodie, J.L., Benner, E]. 8 Kirby W.M.M. (1996) Simplified,
`accurate method for antibiotic assay of clinical specimens. Applied
`Alicrobiology, 14, 1707175.
`Berg, ].N., Scanlan, C.M. 8: Buening, GM. (1984) Clinical models for
`anaerobic bacterial infections in dogs and their use in testing the
`efficacy of clindamycin and lincomycin. American Journal of Veterinary
`Research, 45, 129971306.
`
`@1999 Blackwell Science Ltd, J. vet. Pharmacol. Therap. 22, 2617265
`
`Mean serum clindamycin concentration in dogs 265
`
`
`
`Braden, T.D., Johnson, C.A., Gabel, C.L. et al. (1987) Posologic evaluation
`of clindamycin, using a canine model of posttraumatic osteomyelitis.
`American Journal of Veterinary Research, 48, 1 10171 105.
`Braden. T.D.. Johnson. C.A.. Wakenell. P.
`et
`al,
`(1988) Eificacy of
`clindamycin in the treatment of staphylococcus aureus osteomyelitis in
`dogs. Journal of American Veterinary Medical Association, 192, 1 72171 725.
`Bourne, D.W.A.
`(1986) Multi—forte: a microcomputer program for
`modeling and simulation of pharmacokinetic data. Computer Methods
`Programs Biomedical, 23, 2777281.
`Brown, R.D. & Manno, J.E. (19 78) ESTRIP, a basic computer program for
`obtaining initial polyexponential parameter estimates.
`Journal of
`Pharmacological Science, 67, 1 68 771 69 1.
`Brown, S.A., Zaya, M.J., Dieringer, T.M. et al, (1990) Tissue concentra—
`tions of clindamycin after multiple oral doses in normal cats. Journal of
`Veterinary Pharmacology and Therapeutics, 13, 27072 77.
`Budsberg, S.C.. Gallo, J.M., Starliper, C.E. et al. (1991) Comparison of
`cortical bone local infusion and intravenous administration. Journal of
`Orthopaedic Research, 9, 5947599.
`Budsberg, S.C.. Kemp, D.T. 8: Wolski, N. (1992) Pharmacokinetics of
`clindamycin phosphate in dogs after single intravenous and intra—
`muscular administration. American Journal of Veterinary Research, 53,
`2 3 5 572 3 3 6.
`Dhawan, V.K. 8: Thadepalli, H. (1982) clindamycin: a review of fifteen
`year of experience. Review of Infectious Diseases, 4, 1 13371153.
`Edwards, C.H. & Penney, DE. (1982) Calculus and analytical geometry,
`Englewood Cliffs, Prentice»Hall Inc, NJ.
`Gibaldi, M. (1982) Noncompartmental pharmacokinetics. In Pharmaco—
`kinetics, 211d ed. Marcel Dekker, New York. pp. 409417.
`Greene, CE. (198 9) Antibacterial chemotherapy. In Clinical microbiology
`and infectious diseases in dog and cat. 2nd ed. WB Saunders Co,
`Philadelpia. pp. 4797482.
`Lam, E.C., Himg, C.T., Perrier, D.G. (1985) Estimation of variance for
`harmonic mean half—lives. Journal ofPharmacological Science, 74, 2297231.
`Lavy, E., Ziv. G., Shem—Tov, M. et al. (1999) Oral bioequivalence of
`clindamycin hydrochloride tablets and clindamycin monohydratc
`capsules in normal and fasted dogs. American Journal of Veterinary
`Research, (submitted).
`Panzer, J.D., Brown, D.C., Epstein. W.L. et al. (1972) clindamycin levels
`in various body tissues and fluids. Journal of Clinical Pharmacology, 12,
`2597262.
`the injection site after
`(1980) Tissue damage at
`Rasmussen, F.
`intramuscular injection of drugs in food—producing animals. 111 Trends
`in veterinary pharmacology and toxicology. Eds, van Miert, A.S.J.P.A.M.,
`Frens,
`J., van der Kreck, EW. Elsevier Scientific Publishers,
`Amsterdam. pp. 277330.
`Riviere, J.E. (1988) Veterinary clinical pharmawkinetics modelling. Compen—
`dium for Continuing Education for Practicing Veterinarians, 10, 3147328.
`Stennes. E.. Rasmussen. F.. Svendsen. 0. et al (1978) A comparative
`study of serum creatine phosphokinase ((ZPK) activity in rabbits, pigs
`and humans after intramuscular injection of local damaging drugs.
`Acta Pharmacologica Toxicologia, 42, 35773 64.
`Svendsen, O.
`(1983) Intramuscular injections and local muscle: an
`experimental study of the effect of injection speed. Acta Pharmacologica
`Toxicologia, 52, 3057309.
`\Nebber, D.]., Barbiers, A.R., Lallinger, A.]. et al. (1980) Pharmacoki—
`netics of clindamycin following subcutaneous administration of
`clindamycin phosphate in the canine. Journal of Veterinary Pharmacol—
`ogy and Therapeutics, 3, 1337143.
`Yamaoka, K., Nakagawa, T., Uno, T. (1978) Application of Akaike's
`information criterion (AIC) in the evaluation of linear pharmacokinetic
`equation. Journal of Pharmacokinetics and Biopharmaceutics, 6, 1657175.
`
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