Activation of the Alternative Pathway of Complement by a Phosphorothioate Oligonucleotide: Potential Mechanism of Action

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Vol. 281, Issue 2, 810-816, 1997

Activation of the Alternative Pathway of Complement by a Phosphorothioate Oligonucleotide: Potential Mechanism of Action

Scott P. Henry, Patricia C. Giclas, Janet Leeds, Michael Pangburn, Carol Auletta, Arthur A. Levin and Douglas J. Kornbrust

Department of Toxicology, Isis Pharmaceuticals, Inc. (S.P.H, J.L., A.A.L.), Carlsbad, California, National Jewish Medical & Research Center (P.C.G.), Denver, Colorado, University of Texas, Tyler (M.P.), Tyler, Texas, Huntington Life Sciences (C.A.), East Millstone, New Jersey and Sierra Biomedical, Inc. (D.J.K.), Sparks, Nevada.

	Abstract

Top Abstract Introduction Materials & Methods Results Discussion References

Intravenous infusion of high doses of phosphorothioate oligonucleotides in monkeys has been associated with transient alterationsin hematologic and hemodynamic parameters, which appear to besecondary to complement activation. ISIS 2302, a phosphorothioateoligonucleotide specific for human intracellular adhesion molecule-1,was used to further characterize complement activation in monkeys.Complement activation occurred selectively through the alternativepathway resulting in increased plasma concentrations of the complementsplit products Bb, C3a and C5a. Marked fluctuations in circulatingneutrophil counts and reductions in cardiac output were closelyassociated with peak production of anaphylatoxins C3a and C5a.Changing both dose and infusion duration revealed that complementactivation is related to plasma levels of oligonucleotide, andthat there is a minimum threshold concentration of approximately50 µg/ml of ISIS 2302 that is required to activate complement.Dose regimens in which plasma concentrations do not exceed thisthreshold do not result in complement activation. Further investigationreveals that plasma concentrations of a key regulatory componentof the alternative pathway, Factor H, were also decreased afteradministration of ISIS 2302. Decreases in Factor H levels aresuggestive of a possible mechanism of complement activation. Directinteraction between ISIS 2302 and Factor H was demonstrated ina competition assay, where increasing concentrations of ISIS 2302eluted Factor H from a heparin-sepharose column. These data demonstratea clear correlation between plasma oligonucleotide concentrationsand complement activation. Interactions between ISIS 2302 andFactor H may lead to activation of the alternative complementpathway.

	Introduction

Top Abstract Introduction Materials & Methods Results Discussion References

Phosphorothioate oligonucleotides are designed to hybridize to a specific mRNA, thus inhibiting the expression of a specifictarget gene (Crooke, 1992). Because of Watson and Crick base paringrules, it is possible to make an oligonucleotide that selectivelybinds to a specific mRNA effectively inhibiting protein expressionand, thus, enabling the design of oligonucleotide agents withspecific therapeutic activities. Presently, phosphorothioate oligonucleotidesare being developed as therapeutic agents in human immunodeficiencyvirus, cytomegalovirus, cancer, arthritis, inflammatory boweldisease and organ transplantation (Crooke, 1995; Wagner, 1994).The use of these agents will be dependent on both the therapeuticactivity and their toxicity profile. In this report we documentthe dose-response relationship and the biochemical mechanism ofa phosphorothioate oligonucleotide-mediated toxicity.

The subchronic toxicity of phosphorothioate oligonucleotides has been investigated in rodents and primates (Srinivasan andIversen, 1995), and a pattern of species-specific responses hasbeen characterized that is consistently observed with most compoundsin this class independent of sequence. Several laboratories havedocumented a spectrum of changes in mice and rats that can becollectively characterized as immune stimulation after systemictreatment with phosphorothioate oligonucleotides for several daysor longer (Henry et al., 1996b; Sarmiento et al., 1994). Althoughthere are differences in the quantitative dose-response relationshipfor immune stimulation that appear to be sequence-related, thequalitative similarities in the effects of various phosphorothioateoligonucleotides in rodents are suggestive of some common toxicologicproperties for this class of molecules (Henry et al., 1997).

A somewhat different spectrum of toxicities is induced by phosphorothioate oligonucleotides in nonhuman primates. Clinicalobservations in monkeys (i.e., macaques) given large systemicdoses include transient lethargy, periocular edema, susceptibilityto bruising and acute mortality (Cornish et al., 1993; Galbraithet al., Henry et al., 1996a). Further investigation in instrumentedanesthetized animals revealed pronounced hemodynamic alterations,including central hypotension and reductions in cardiac outputthat were associated with activation of complement (Galbraithet al., 1994). Although other studies have described complementactivation associated with administration of phosphorothioateoligonucleotides (Galbraith et al., 1994), this study fully characterizesthe dose-response relationship and the pattern of complement splitproduct formation. The objective of this study was to furthercharacterize the relationship between plasma concentration ofphosphorothioate oligonucleotides and complement activation, toestablish safe plasma levels of oligonucleotide and to definea potential mechanism of complement activation. The data obtained,particularly the existence of a threshold concentration for complementactivation, are highly relevant to the continued safe use of phosphorotioateoligonucleotides.

	Materials and Methods

Top Abstract Introduction Materials & Methods Results Discussion References

Test material. ISIS 2302 (M_r = 6781) is a 20-base phosphorothioate oligonucleotide (5 $'$ -GCCCAAGCTGGCATCCGTCA-3 $'$ ) with a sequence that is complementaryto a 3 $'$ -untranslated region of the human intracellular adhesionmolecule-1 mRNA. ISIS 2302 was synthesized by Isis Pharmaceuticals(Carlsbad, CA) (purity >92% full-length oligomer). ISIS 2302 wasformulated in phosphate-buffered saline (pH 7.4) at a concentrationof 4 mg/ml.

Animals. Fifteen female cynomolgus monkeys (Worldwide Primates, Inc., Miami, FL) were randomly chosen and assigned to dose groups basedupon body weight. Body weight ranged from 2.5 to 3.5 kg, but theexact age was unknown. Monkeys were housed in elevated metal gridcages and were maintained in an environmentally controlled room(12-hr light/dark cycle) with ad libitum access to water. Theamount of food presented each day was approximately 4% of themean body weight for all animals in the room. All animal husbandryprocedures were in full compliance with AAALAC guidelines.

Study design. Monkeys received single doses of 2, 3.3, 6.6, 10 or 20 mg/kg of ISIS 2302 or a vehicle control solution by i.v. infusion forperiods ranging from 2 to 120 min (N = 3-4 per group). Some monkeyswere used repeatedly (up to 5 separate treatment regimens) forevaluation of acute toxicity after a 2-week wash out period. Monkeyswere observed continuously for the first several hours after treatmentto document acute clinical signs of toxicity. Blood samples wereobtained at various intervals throughout the dosing or monitoringperiods in order to evaluate plasma concentrations of ISIS 2302and potential complement activation or alterations in hematologyparameters.

Hemodynamic evaluation. Alterations in mean arterial pressure, heart rate and cardiac output were assessed after a 10-min infusion of 20 mg/kg ofISIS 2302 in ketamine-anesthetized monkeys. A catheter was placedin the femoral artery for recording central pressure and heartrate. A Swan Ganz catheter was placed in the right atrium fordetermination of cardiac output by the thermal dilution method.ECG recordings were also obtained during this period. Continuouson-line monitoring was performed during the infusion and for 1to 2 hr after using a MACLAB (FID Instruments, Castle Hill, Australia)computerized multichannel chart recording system.

Analysis of complement activation. The level of complement split products Bb, C3a_{des arg,} C4a_{des arg} and C5a_{des arg} was determined in EDTA plasma samples usingcommercially available radioimmunoassay or enzyme-linked immunosorbentassay kits. C3a_{des arg}, C4a_{des arg} and C5a_{des arg} were measuredusing a radioimmunoassay kit from Amersham Life Sciences (Amersham,Little Chalfont, Buckinghamshire, England). The Bb fragment ofFactor B was determined using an enzyme immunoassay from Quidel(San Diego, CA).

Total hemolytic complement activity in serum (CH50) was assayed in serum samples using the standard hemolytic assay (Harbeckand Giclas, 1991

). Factor H concentrations in monkey plasma weredetermined by radial immunodiffusion (Harbeck and Giclas, 1991

)using an anti-human Factor H antibody that cross-reacts stronglywith monkey Factor H.

Factor H binding assay. The relative affinity of Factor H for heparin [Sigma Chemical Co. (St. Louis, MO); M_r = 16,000-17,000] and ISIS 2302 was estimatedin a competitive binding assay as described previously (Pangburnet al., 1991). Radiolabeled Factor H was bound to a heparin-sepharosesolid-phase column. Solutions containing increasing concentrationsof heparin or ISIS 2302 were added to the column. Column eluateswere analyzed to determine the amount of Factor H eluted.

ISIS 2302 analysis. Plasma concentrations of intact ISIS 2302 were determined from EDTA plasma using capillary gel electrophoresis and UV detection(Leeds et al., 1996). Separation and resolution of intact ISIS2302 and its metabolites were obtained using polyacrylamide gel-filledcolumns under denaturing conditions (7 M urea). Quantitation wasbased on the UV absorbance at 260 nm of ISIS 2302 peaks relativeto an internal standard.

	Results

Top Abstract Introduction Materials & Methods Results Discussion References

Complement activation and physiological response. Intravenous infusion of 20 mg/kg of ISIS 2302 over 10 min results in strong activation of the complement cascade as indicatedby a reduction in CH50 activity and an increase in the biologicallyactive split products C3a and C5a over time (fig. 1, A and B)(Hugli and Muller-Eberhard, 1978). The 60% decrease in total hemolyticcomplement activity, CH50, suggests extensive complement activation.In addition to the appearance of the anaphylatoxins C3a and C5a,there was a marked increase in Bb, but no significant change inthe marker for the classical pathway, C4a (fig. 1A). C3a and C5aare common to both classical and the alternative pathway activation,whereas the complement split product Bb is formed only as a resultof the activation of the alternative pathway. Thus, the increasesin Bb and unchanged levels of C4a indicate that only the alternativepathway is activated in cynomolgus monkeys by treatment with ISIS2302.

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Fig. 1. A representative pattern of complement split products generated by a 10-min i.v. infusion of 20 mg/kg of ISIS 2302 in a cynomolgusmonkey. A: Plasma concentrations of C5a, C3a and Bb were increased;however, no increase in C4a split product was evident relativeto plasma concentrations before treatment. Peak concentrationsof complement split product were C3a = 199 ng/ml; C5a = 74.9 ng/ml;Bb = 4.03 µml; C4a = 225 ng/ml. B: The extent of complement activationafter this dose resulted in a 60% reduction in the total hemolyticcomplement activity. The temporal relationship between dosingand complement activation is very consistent among animals andis correlated with peak plasma concentrations of oligonucleotide.Although the pattern of split products is similar for all animals,the absolute amount of split products generated will vary dependingon individual animal sensitivity to complement activation.

Because the appearance of Bb in plasma is characteristic of the alternative pathway, and it is more long-lived in plasma thanthe other split products measured in these experiments (fig. 1A),we selected Bb as a marker of complement activation for subsequentstudies reported herein. The relative stability of Bb in plasmaincreased the probability of detecting complement activation evenwith limited sampling periods.

In addition to complement activation, i.v. infusion of 20 mg/kg of ISIS 2302 over 10 min in monkeys was associated with anumber of other physiologic responses, including alterations inhematologic and hemodynamic parameters. Based on the apparenttemporal relationship of these changes to dosing and C5a production,and the known biological effects of the C5a anaphylatoxin, itis possible that these changes were secondary to complement activation.Specifically, fluctuations in circulating neutrophil counts occurredthat were characterized by a marked but transient neutropenia,followed by rebound neutrophilia (fig. 2). These effects on neutrophilcounts, particularly the neutropenic phase, were highly correlatedwith increases in C5a levels (compare figs. 1A and 2). The peakplasma concentrations of C5a at 10 min (i.e., end of infusion)were coincident with the maximal decrease in neutrophil counts(i.e., 10-20 min). As C5a levels returned toward base line, neutrophilsreturned to predose levels. However, neutrophil counts continuedto increase, reaching a maximum concentration that was several-foldabove base-line values. Neutrophil counts peaked approximately1 hr after the start of infusion and returned toward base lineby 4 to 6 hr. Neutrophilia was also associated with increasesin nonsegmented (presumably immature) neutrophils (fig. 2).

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Fig. 2. A representative pattern of hematology changes generated by a 10-minute i.v. infusion of 20 mg/kg of ISIS 2302 in a cynomolgusmonkey. Transient neutropenia followed by a rebound neutrophiliareflect complement activation and the production of C5a. Neutrophiliaat later time points is associated with increases in circulatingnonsegmented neutrophils (insert). Data represented in this figurewere obtained from the same animal as depicted in figure 1. Neutropeniais consistently associated with increased levels of C5a.

Alterations in hemodynamic parameters were also temporally related to complement activation. MAP increased slightly 5 mininto the infusion, followed by a rapid and profound decrease inMAP (fig. 3). MAP decreased from a base-line level of approximately80 to 25 mm Hg within 20 min. The initiation of these hemodynamicchanges correlated with peak levels of C5a and the neutropenicresponse. Blood pressure remained low through the monitoring period,with an increasing trend toward base line. Heart rate decreasedin parallel with the decline in MAP, falling from 170 to approximately80 beats/min between 6 and 14 min of the monitoring period (fig.3). Heart rate returned to base-line levels approximately 30 minafter the end of infusion. In addition, similar dose regimenswere occasionally associated with clinical observations includingdecreased activity level (i.e., lethargy) and periocular swellingin monkeys (data not shown).

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Fig. 3. A representative pattern of hemodynamic changes after a 10-min i.v. infusion of 20 mg/kg of ISIS 2302 in a ketamine-anesthetizedcynomolgus monkey. Blood pressure increased slightly and decreasedin parallel with heart rate near the end of the infusion period.Data represented in this figure were obtained from the same animalas depicted in figure 1. The temporal relationship between dosingand hemodynamic effects is again consistent among animals. Thepresence and severity of hemodynamic effects, however, vary greatlyamong animals and are roughly correlated with the extent of C5aincrease. Many animals experienced no hemodynamic alterations.

Dose-response relationship. To assess the role of peak plasma concentrations in the activation of complement, a series of infusions of varying lengthwere performed. Keeping the dose constant and increasing the durationof infusion from 10 to 60 min resulted in a marked decrease inthe amount of Bb produced (fig. 4). The peak concentration ofBb after a 10-min infusion of 10 mg/kg was 13 µg/ml (fig. 4).By comparison, 30- and 60-min infusions of 10 mg/kg yielded lowerpeak Bb levels of 3.25 and 1.5 µg/ml, respectively. Decreasingthe dose in a 60-min infusion from 10 to 6.6 mg/kg also resultedin a further decrease in Bb split product formation, indicatingthe dose-dependent nature of this response. Plasma concentrationsof Bb were proportional to plasma ISIS 2302 concentrations atthe end of infusion, with higher plasma concentrations resultingin greater complement activation. Doses of 6.6 mg/kg infused over60 min were considered to be noncomplement activating becauseBb levels did not exceed the normal range of variability (fig.4).

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Fig. 4. The amount of Bb produced after i.v. infusion of ISIS 2302 was dependent on dose and rate of infusion. Peak levels of Bb decreasedas the dose was lowered or the duration of infusion was extended.There were a number of dose regimens that did not result in complementactivation. The values represent mean values of at least 3 animals± S.E. (The dashed line represents the upper limit in the normalrange of variability.)

Other dose regimens that did not result in increased Bb levels were 6 mg/kg over 120 min, 3.3 mg/kg over 60 min and 2 mg/kgover 10 min (data not shown). In addition to Bb, C5a was measuredafter these dose regimens and also found to be unaffected, thusconfirming the absence of complement activation. These data indicatethat at appropriate infusion rates and doses ISIS 2302 can beadministered by i.v. infusion without activating complement andimply that complement activation is related to plasma C_max (table1).

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TABLE 1
Peak plasma concentration of ISIS 2302 after various dose regimens

A clear pattern is observed when Bb concentrations are plotted as a function of plasma ISIS 2302 concentrations during infusion(fig. 5). With increasing plasma concentrations of ISIS 2302,there is little or no increase in Bb concentration until plasmaconcentrations exceed 50 µg/ml. Above this concentration the complementcascade appears to be activated and there is an abrupt increasein Bb. These data clearly demonstrate a plasma threshold concentrationfor Bb production. When plasma concentrations remained at or below50 µg/ml during the infusion there were no increases in Bb levelsand, by inference, no complement activation (fig. 5). However,at concentrations above 50 µg/ml, complement activation and Bbproduction were consistently observed.

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Fig. 5. An ISIS 2302 plasma concentration threshold for complement activation. Concentrations of ISIS 2302 are plotted against thecorresponding concentration of Bb produced during i.v. infusion.This figure represents data obtained during the course of infusionfrom over 50 animals, and ranging from 2 to 20 mg/kg infused from10 to 120 min. (The dashed line represents the normal range ofvariability in plasma Bb in cynomolgus monkeys.)

Effects of ISIS 2302 on the APC. Factor H is a plasma protein that plays a key role in regulating amplification of the alternative pathway and has previouslybeen identified as a DNA-binding protein (Gardner et al., 1980b).Monkeys treated with 10 mg/kg of ISIS 2302 infused over 10, 30or 120 min had a dose-dependent and infusion time-dependent decreasein plasma Factor H levels that were closely correlated with increasingplasma concentrations of ISIS 2302 throughout the infusions (fig.6). In contrast to the pattern of a threshold plasma concentrationeffect on complement activation and Bb production, a linear concentrationresponse was observed on plasma Factor H concentrations. Smalldecreases in Factor H levels were also observed after doses thatdid not result in complement activation. Decreases in plasma FactorH were dependent upon both dose and plasma concentrations of ISIS2302. Furthermore, the decrease in Factor H was proportional tothe levels of Bb produced during complement activation. PlasmaFactor H concentrations stabilized and began to return towardbase-line levels after the end of infusion (fig. 6).

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Fig. 6. Intravenous infusion of ISIS 2302 causes a decrease in the circulating plasma concentrations of Factor H. A: Decreases inconcentrations of Factor H were dependent on infusion time andwere lowest at the end of infusion. B: Peak plasma concentrationsof ISIS 2302 occur at the end of infusion and correspond to themaximal decrease in Factor H. The values represent mean valuesof at least 3 animals ± S.E.

In order to characterize further the interaction between ISIS 2302 and Factor H, we examined direct interactions between ISIS2302 and factor H. In competitive binding experiments, radiolabeledFactor H was bound to a heparin-sepharose column and eluted withbuffers containing increasing concentrations of heparin or ISIS2302. Both polyanions (heparin and ISIS 2302) could elute FactorH from the solid support (fig. 7). The concentrations of polyanionrequired to elute 50% of Factor H were 20 µg/ml of ISIS 2302 and4.5 µg/ml of heparin (i.e., 2.9 and 0.27 µM, respectively). Thisapparent difference in affinity may be attributed to the muchgreater electronegativity of heparin. If the elution of FactorH is dependent on the total net negative charge, the 10-fold differencein the molar elution concentrations may not represent a dramaticdifference in binding affinity. Nevertheless, these results indicatea relatively strong interaction between ISIS 2302 and Factor H.

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Fig. 7. In a competition-binding assay, ISIS 2302 was able to elute Factor H from a solid support. Increasing concentrations of heparinand ISIS 2302 resulted in a concentration-dependent elution ofradiolabeled Factor H from a heparin-sepharose column. The concentrationrequired to elute 50% of Factor H was 20 µg/ml for ISIS 2302 and4.5 µg/ml for heparin (2.9 and 0.27 µm, respectively).

	Discussion

Top Abstract Introduction Materials & Methods Results Discussion References

Intravenous administration of high doses of ISIS 2302, as well as other phosphorothioate oligonucleotides, results in complementactivation in monkeys (Galbraith et al., 1994). In this studywe further characterized the profile of complement split productsformed in ISIS 2302-treated animals and determined that the alternativepathway was selectively activated, as indicated by increases inBb concentrations and the lack of any increase in the classicalpathway marker, C4a. Close examination of the temporal relationshipbetween the production of the anaphylatoxins, C3a and C5a, andother acute alterations suggests that changes in hematologic andhemodynamic parameters observed in monkeys after phosphorothioateoligonucleotide administration may be secondary to complementactivation. Some of these alterations, particularly the fluctuationsin neutrophil counts described above, are characteristic of exposureto C5a. C5a has been shown to bind to specific receptors of neutrophilstriggering a series of intracellular events resulting in increasedexpression of surface adhesion molecules and a loss of deformability(Frank and Fries, 1991; Kajita and Hugli, 1990). This activationoccurs rapidly and leads to sequestration of neutrophils in capillarybeds (Kajita and Hugli, 1990). As C5a is cleared from plasma,neutrophils regained their deformability and return to circulation.In addition, the chemotactic influence of C5a causes recruitmentof immature neutrophils (nonsegmented neutrophils) from bone marrow,resulting in rebound neutrophilia (Ember et al., 1992). This patternof changes in circulating neutrophil counts was observed in monkeystreated with ISIS 2302 and has been reported for monkeys treatedwith other phosphorothioate oligonucleotides (Galbraith et al.,1994). Shortly after oligonucleotide administration, a pronounceddrop in circulating neutrophils occurred that was closely associatedin time with the formation of C5a. Subsequently, there was a reboundneutrophilia that largely consisted of immature (presumably bonemarrow-derived) neutrophils. These changes in neutrophil countswere not observed in the absence of complement activation. Repeatedadministration of ISIS 2302 either daily or every other day neitherenhanced nor diminished the activation of complement and therewas no evidence of cumulative effects after a series of doses(data not shown).

In addition to their effects on neutrophils, the anaphylatoxins (C3a and C5a) have been reported to activate other cell typesincluding mast cells and basophils (Hugli and Muller-Eberhard,1978), which can lead to release of vasoactive autocoids (e.g.,histamine, prostaglandins, leukotrienes, etc.). These, or other,vasoactive agents may also be released from endothelial cellssubsequent to their interaction with activated neutrophils. Suchmediators may cause changes in vascular permeability and tone,and could be responsible for the hypotension that occurs in ISIS2302-treated monkeys after doses that activate the complementsystem. It is also conceivable that other acute clinical observationsassociated with ISIS 2302 administration (i.e., transient lethargyand periocular swelling) were secondary manifestations of complementactivation. Activation of the complement system has been reportedto occur in a number of diverse but commonly used clinical proceduresincluding extracorporeal blood processing (e.g., hemodialysis),drug treatment (e.g., sulfonamides, corticosteroids, dextrans,heparin and protamine sulfate), high-dose treatment with immunoglobulins(e.g., i.v. immunoglobulin treatment) or treatment with certainrecombinant proteins (e.g., interleukin-2 and tissue plasminogenactivator) (Svehag, 1991).

Plasma concentrations of ISIS 2302 can be used to predict the extent of complement activation based on the relationship definedin these studies. We have identified a threshold concentrationof 50 µg/ml for ISIS 2302, below which no complement activationwas detected. At higher plasma levels of ISIS 2302, the relativeamounts of split products formed were generally related to peakplasma concentration and, to some extent, to the duration of timethat the plasma levels remained elevated. Decreasing peak plasmalevels of ISIS 2302 by lowering the dose or prolonging the durationof i.v. infusion while holding the dose constant resulted in loweramounts of complement split products generated. The incidenceand severity of hematologic and hemodynamic disturbances in themonkeys appeared to be closely associated with the amount of complementsplit products generated, especially C5a, which is consistentwith dose-dependent effects of C5a on neutrophil counts and physiologicalresponses in vivo and neutrophil morphology in vitro (Ehrengruberet al., 1994). In our studies, hemodynamic effects in monkeyswere observed at plasma ISIS 2302 concentrations of 90 µg/ml orhigher, whereas the threshold for complement activation was 50µg/ml. At concentrations of ISIS 2302 in the plasma above 90 µg/ml,Bb levels were more substantially elevated compared to plasmaISIS 2302 concentrations between 50 and 90 µg/ml, and thus wouldcorrelate with increased anaphylatoxin levels. Anaphylatoxinsare the known biological mediators of complement activation andthe markedly elevated levels observed with some of the dose regimensin this study could explain the changes in hemodynamic parameters.

That the alternative pathway was activated in the absence of classical pathway activation has important implications on thepotential mechanism of activation. The APC is involved in recognitionand destruction of foreign organisms (Tomlinson, 1993). Generally,this pathway is thought to require some type of activating surfaceto initiate the cascade, such as virus-infected cells, bacteriaor parasites (Pangburn and Muller-Eberhard, 1984). The alternativepathway is considered to be constitutively active and amplificationof the pathway under normal conditions is suppressed by the combinedaction of a number of negative regulatory components includingFactor H and Factor I. Thus, Factor H and Factor I are importantregulatory components of the alternative pathway. Factor H bindsto the BbC3b complex and displaces the Bb, thus providing a bindingsite for Factor I that cleaves C3b to iC3b, therefore preventingfurther interaction with Factor B, which would lead to the formationof the C3b convertase and ultimately to full amplification ofthe pathway (Pangburn and Muller-Eberhard, 1984). Under conditionsof activation (e.g., exposure to bacteria) the affinity of FactorH and Factor I for C3b bound to the activating surface is dramaticallyreduced by the binding of properdin, thus eliminating down-regulationof the pathway and allowing amplification of the complement cascadesubsequent to formation of the C3bBb convertase. If oligonucleotidetreatment alters the activity or concentration of these regulatoryproteins, this could be the stimuli for alternative pathway activation(Meri and Pangburn, 1990).

The APC is a relatively simple system composed of only six plasma glycoproteins (C3 and Factors B, D, H, I and P) (Schreiberet al., 1978). Two of the components of the alternative pathway,Factor H and Factor B, have been previously identified as DNA-bindingproteins (Gardner et al., 1980a,b). A specific interaction betweenFactor H and ISIS 2302 was demonstrated herein by the abilityof the oligonucleotide to compete for a binding site on FactorH and to elute the radiolabeled protein from a heparin-sepharosecolumn.

Intravenous administration of ISIS 2302 to monkeys resulted in decreases in plasma Factor H levels. Elimination of FactorH from plasma could theoretically lead to disregulation of theAPC, because Factor H plays an important role in down-regulatingthe alternative pathway activity (Pangburn and Muller-Eberhard,1984). In studies where the alternative pathway has been reconstitutedfrom purified components, it was demonstrated that regulatoryfunction was compromised when Factor H concentrations were reducedbelow 50% of base-line levels (Schreiber et al., 1978). Therefore,decreases in plasma concentrations of Factor H after high dosesof ISIS 2302 likely resulted in the loss of alternative pathwayregulation. This relationship between Factor H levels and alternativepathway activation may explain the apparent threshold for complementactivation in that regulation of the pathway is only compromisedwhen enough Factor H has been removed from circulation.

Activation of the alternative pathway through loss or removal of Factor H from the plasma has been demonstrated in vitro.Dextran-sulfate linked to insoluble sepharose particles was shownto sequester Factor H from the fluid phase, resulting in alternativepathway activation in vitro (Bitter-Suermann et al., 1981). Inaddition, immunoprecipitation of Factor H from normal serum usinganti-Factor H antibodies resulted in rapid activation of the alternativepathway (Boackle et al., 1983). Although it appears that depletionof Factor H in plasma resulted in complement activation, it isnot clear from these experiments how ISIS 2302 treatment in monkeysleads to the reduction of Factor H levels.

Complement activation by a phosphorothioate oligodeoxynucleotide is not unique to the ISIS 2302 sequence or length (20 nucleotides)and has been observed for a number of oligonucleotides (S. P.Henry, unpublished data), including the human immunodeficiencyvirus-rev antisense compound mentioned previously (25 nucleotides)(Galbraith et al., 1994). Thus, complement activation appearsto be largely independent of sequence and more attributable toexposure to the chemical class. Due to the nonspecific natureof this interaction, it is likely that the larger chain-shortenedmetabolites (possibly down to 16 nucleotide molecules) may alsocontribute to complement activation and, therefore, should alsobe taken into consideration when defining exposure.

Results of these studies indicate that complement activation resulting from i.v. infusion of phosphorothioate oligonucleotidesis related to peak plasma concentrations of oligonucleotide, andthat there is a threshold concentration for activation. Becauseseveral of the acute toxicities associated with phosphorothioatetreatment, including hemodynamic alterations and neutrophil fluctuations,appear to be secondary to complement activation, this thresholdfor activation is important for continued safe dosing of thesecompounds. The cause of alternative pathway activation appearsto be due to reduced levels of plasma Factor H, thus allowingunregulated amplification. The inability to establish an in vitroassay for complement activation has prevented us from determiningif this effect of phosphorothioate oligonucleotides in monkeysis relevant to humans. However, complement activation is not expectedto occur in humans, as the highest doses of ISIS 2302 that arecurrently being used in the clinic produce peak plasma concentrationsof oligonucleotide that are 4- to 5-fold lower than the thresholdfor activation (J. Glover, submitted). Identification of the molecularmechanism for complement activation will facilitate the designof future generations of antisense oligonucleotides that havedecreased potential for these acute toxicities.

	Footnotes

Accepted for publication January 21, 1997.

Received for publication August 7, 1996.

Send reprint requests to: Scott P. Henry, Ph.D., Department of Toxicology, Isis Pharmaceuticals, Inc., 2292 Faraday Ave., Carlsbad, CA 92008.

	Abbreviations

APC, alternative pathway of complement; mRNA, messenger ribonucleic acid; C_max, maximum plasma concentration; MAP, mean arterial pressure.

	References

Top Abstract Introduction Materials & Methods Results Discussion References

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				J. P. Sheehan and H.-C. Lan Phosphorothioate Oligonucleotides Inhibit the Intrinsic Tenase Complex Blood, September 1, 1998; 92(5): 1617 - 1625. [Abstract] [Full Text] [PDF]

				R. Morishita, J. Higaki, N. Tomita, and T. Ogihara Application of Transcription Factor "Decoy" Strategy as Means of Gene Therapy and Study of Gene Expression in Cardiovascular Disease Circ. Res., June 1, 1998; 82(10): 1023 - 1028. [Abstract] [Full Text] [PDF]