Introduction
Complement-mediated cytotoxicity plays a central role in the pathogenesis of seropositive neuromyelitis optica spectrum disorders (herein called NMO), in which immunoglobulin G autoantibodies against water channel aquaporin-4 (AQP4), called AQP4-IgG, bind to astrocytes in brain, spinal cord and optic nerve [
9,
10]. Following astrocyte injury, downstream inflammation, blood-brain barrier disruption and potentially additional mechanisms result in oligodendrocyte injury and demyelination [
11,
17,
29]. Optic neuritis and transverse myelitis are the major clinical manifestations of NMO, which can produce visual and motor impairment, and brain involvement can occur as well. Though AQP4 is expressed in some peripheral organs outside of the central nervous system, including skeletal muscle, kidney and stomach [
8,
19], these organs are rarely affected in NMO, with only a few reports of NMO-associated myositis associated with elevated creatine phosphokinase and skeletal muscle pathology [
7,
13,
27].
It has been unclear why peripheral AQP4-expressing cells, which are exposed to high levels of circulating AQP4-IgG in seropositive NMO, are largely spared. Rodent studies show prompt deposition of circulating AQP4-IgG on peripheral AQP4-expressing cells [
1,
20], and humans can be AQP4-IgG seropositive for many years prior to clinical manifestations of NMO [
16]. Rodents administered AQP4-IgG systemically do not spontaneously develop pathological changes in the central nervous system or in peripheral organs, though pathology in brain is seen following mechanical disruption of the blood-brain barrier [
1].
Here, we tested the hypothesis that complement regulator protein CD59 is responsible for protection of AQP4-expressing peripheral cells in seropositive NMO. CD59 is a phosphoinositol-linked membrane glycoprotein that inhibits formation of the complement terminal membrane attack complex [
6,
21,
26,
34]. The motivation for this work is the expression of CD59 in AQP4-expressing cells in the central nervous system and in the periphery, and our prior data showing that CD59
−/− mice are highly sensitive to development of NMO pathology following direct administration of AQP4-IgG and human complement into brain or cerebrospinal fluid [
33]. CD59
−/− rats also develop marked brain and spinal cord pathology following direct AQP4-IgG administration [
32], albeit without the need for coadministration of complement, because rats, unlike mice, have an active classical complement system [
2,
22]. We report here marked injury to skeletal muscle following systemic AQP4-IgG administration to CD59
−/− rats, offering an explanation for the sparing of peripheral organs in seropositive NMO.
Materials and methods
Materials
Purified recombinant AQP4-IgG (rAb-53) [
3,
5] was provided by Dr. Jeffrey Bennett (Univ. Colorado, Denver) and (non-NMO) pooled human IgG, as control, was purchased from Pierce Biotechnology (Rockford, IL). Some studies were done using an antibody fragment-based complement inhibitor, herein called Comp
inh (to be reported separately), which inhibits serum complement activity by >95% for 8–12 h after intravenous administration. Unless otherwise specified chemicals were purchased from Sigma-Aldrich (St. Louis, MO).
CD59−/− rats
CD59
−/− rats in a Sprague-Dawley background were custom-generated by Transposagen Biopharm. Inc. (Lexingtobon, KY) using CRISPR-Cas9 gene targeting technology as described [
32]. In vivo studies were done on 8- to 10-week-old, weight-matched CD59
+/+ and CD59
−/− rats. Rats were maintained in air-filtered cages and fed normal rat chow in the University of California, San Francisco (UCSF) Animal Care facility. All procedures were approved by the UCSF Committee on Animal Research (approval number AN108551).
Blood and urine analysis
Blood (800 μL) was collected before and 24 h after AQP4-IgG injection. Hematological parameters were measured using a Genesis Hematology Analyzer (Oxford Science, Oxford, CT) in which 80 μL blood was collected into a MiniCollect tube with EDTA (Greiner Bio-One GmbH, Kremsmunster, Austria). Serum was obtained by collection of blood in 1.5-ml Eppendoff tubes then allowing clotting for 30 min followed by centrifugation at 800 g for 10 min at 4 °C. Serum was frozen at −70 °C for blood chemistry analyses (IDEXX BioResearch, Sacramento, CA). Urine was collected for determination of osmolality using a freezing-point depression osmometer (Model 3320 Osmometer, Advanced Instruments Inc., Natick, MA).
AQP4-IgG pharmacokinetics
Adult CD59+/+ and CD59−/− rats were administered AQP4-IgG (4 mg/kg body weight in PBS) by intraperitoneal injection in a total volume of 500 μL. Blood was collected through the tail vein at 1, 2, 4, 6, 8, 24 and 48 h, left for 30 min at room temperature to allow clotting, and centrifuged for 10 min at 800 g at 4 °C. Serum was diluted 50,000-fold and human IgG concentration was determined using a human IgG ELISA kit (GenWay, San Diego, CA).
Intraperitoneal injection model
AQP4-IgG or (non-NMO) control human IgG (5 mg/kg body weight) was injected intraperitoneally. At 24 h, clinical motor scores were recorded, as adapted from scoring used for neuroinflammation models in rodents [
18]: score 0, normal movement; score 1, tail paralysis; score 2, hindlimb paralysis; score 3, hindlimb and frontlimb paresis with breathing difficulty; score 4, complete paralysis with moribund condition. Then rats were deeply anesthetized using ketamine (100 mg/kg) and xylazine (10 mg/kg) and transcardially perfused with 200 mL heparinized PBS and 200 mL of 4% PFA in PBS. Brain, optic nerve, spinal cord (cervical), skeletal muscle, kidney and stomach were removed and post-fixed for 4 h in 4% paraformaldehyde (PFA) and cryoprotected in 20% sucrose. Tissues were embedding in OCT compound and sectioned at 7-μm thickness using a cryostat (CM1900, Leica) for immunofluorescence. For complement inhibition studies, Comp
inh (50 mg/kg) was injected intravenously just before and 12 h after intraperitoneal AQP4-IgG (or control IgG) administration.
Immunofluorescence
Frozen sections of harvested tissues were immunostained as described [
32]. Briefly, sections were incubated in blocking solution (1% BSA containing 0.3% Triton X-100 in PBS) for 1 h at room temperature, then incubated overnight at 4 °C with primary antibodies against AQP4 (1:200, Santa Cruz Biotechnology), human IgG (1:200, Santa Cruz Biotechnology), C5b-9 (1:100, Hycult Biotech, PA), CD45 (1:50, Cambridge, MA), CD59 and CD55 (1:50, LSBio, Seattle, WA), CD46 (1:50, Abcam, MA), GFAP (1:200; Millipore), ionized calcium binding adaptor molecule 1 (Iba1; 1:400, Wako, Richmond, VA), or myelin basic protein (MBP, 1:100, Santa Cruz Biotechnology), followed by the appropriate species-specific Alexa Fluor-conjugated secondary antibody for 1 h (5 μg/mL each, Invitrogen) at room temperature. Sections were mounted with Prolong Gold antifade reagent with DAPI (Invitrogen, Life Technologies, Eugene, OR) for visualization of immunofluorescence on a Leica fluorescence microscope or Nikon confocal microscope.
Statistics
Data are presented as mean ± S.E.M. Statistical analysis was performed using Prism 5 GraphPad Software package (San Diego, CA). The normality of the data was established by Bartlett’s test for equal variances and a one-way ANOVA with Newmann-Keuls post-hoc test to compare groups.
Discussion
The principal finding here is that rats lacking complement inhibitor protein CD59 develop marked weakness and pathological changes in AQP4-expressing skeletal muscle following systemic administration of AQP4-IgG, whereas under identical conditions wildtype rats do not. Mild pathological changes were also seen in AQP4-expressing epithelial cells in the renal inner medullary collecting duct, but not in AQP4-expressing gastric parietal cells. Injured AQP4-expressing cells in skeletal muscle of CD59−/− rats showed reduced AQP4 expression, deposition of activated complement, and inflammation. Skeletal muscle injury was associated with marked elevation in serum creatine phosphokinase, which was largely prevented by complement inhibition, supporting the conclusion that complement-dependent cytotoxicity is responsible for peripheral organ injury in the seropositive CD59−/− rats. The absence of demonstrable brain or spinal cord injury suggests that the marked motor dysfunction seen by 24 h is the consequence of acute skeletal muscle injury rather than central nervous system injury. Respiratory failure because of diaphragmatic involvement may have contributed to the early mortality. The study here required CD59−/− rats rather than mice because of the low activity of mouse complement, precluding the use of mice to study the consequences of systemic AQP4-IgG seropositivity.
There are a few reports of NMO myositis with elevated serum CK, though no reports of NMO-associated pathology in other AQP4-expressing peripheral organs. In a report of 2 seropositive NMO patients with diffuse myalgias, a substantial transient elevation of CK was found, with muscle biopsy showing reduced AQP4 expression and deposition of activated complement [
13], similar to the pathological changes seen in seropositive CD59
−/− rats here. One case of CK elevation at the time of NMO attacks was reported, but without muscle findings [
7]. In a retrospective study of 733 cases of NMO in Japan, three patients were found with CK elevation and general fatigue weeks before symptoms of optic neuritis [
27]. Though renal disease has not been reported in NMO, perhaps some patients manifest a mild urinary concentrating defect, as found in AQP4 knockout mice [
12], and perhaps urinalysis might reveal cellular evidence of collecting duct injury.
Our findings support the conclusion that peripheral organ injury is largely absent in seropositive NMO because of protection by CD59 against complement-mediated injury in AQP4-expressing cells. Perhaps the myositis seen in a very small number of NMO patients is caused by altered CD59 expression or CD59 polymorphisms, though this possibility has not been investigated. It would also be interesting to study the expression of CD59 and other complement regulator proteins in central nervous system and peripheral organ in human NMO. The apparent greater sensitivity of skeletal muscle to complement-induced injury, compared with other AQP4-expressing peripheral organs, might be related to the greater metabolic activity of skeletal muscle cells, or perhaps to differences in the expression of other complement inhibitors. Our results also support the central role of CD59 in the modulation of AQP4-IgG-initiated complement injury and hence suggest the potential therapeutic benefit in NMO of upregulation of astrocyte CD59 or alternative complement regulator proteins by pharmacological or other means.
Previously, various explanations have been offered for the general absence of NMO disease in peripheral, AQP4-expressing organs. Once set of explanations focus on AQP4, postulating that differences in AQP4 expression, localization or membrane clustering affect AQP4-IgG binding and consequent complement activation [
14,
25]. However, the robust binding of AQP4-IgG to peripheral AQP4-expressing cells in rodents argues strongly against an AQP4-centric explanation, as do AQP4 biochemical and freeze-fracture electron microscopy studies [
19,
23,
30,
31]. AQP4-IgG is deposited in skeletal muscle where it has been studied in seropositive humans [
13], and AQP4-IgG is rapidly deposited in multiple AQP4-expressing peripheral organs following its systemic delivery to rodents [
1,
20]. Another possible explanation for sparing of peripheral organs in NMO is the unique milieu of the central nervous system, which, unlike peripheral organs, might amplify an inflammatory response because of the presence of microglia, a narrow extracellular space, and a blood-brain barrier that impedes inflammatory cell exit. However, there is no experimental evidence to support this explanation.
The findings here raise the question of why CD59 in astrocytes does not fully protect against AQP4-IgG/complement injury as it appears to do in peripheral organs. Our prior data using mouse and rat models of NMO produced by injection of AQP4-IgG into brain or the spinal cerebrospinal space implicate a protective role for CD59 in brain and spinal cord in vivo [
32,
33], which was supported by in vitro data in astrocyte cultures from knockout mice and rats or following CD59 enzymatic neutralization. Saadoun and Papadopoulos [
24] reported that complement inhibitors, including CD59, are not protective against complement injury in CNS tissues. Though this conclusion is not supported by our findings in CD59
−/− rats and mice, they reported interesting immunofluorescence in mouse brain in which CD59 expression was seen on astrocyte cell bodies but not on AQP4-rich foot-processes near microvessels. We believe that higher-resolution imaging studies using electron microscopy or super-resolution fluorescence microscopy are needed to resolve unambiguously the subcellular localization of CD59 and AQP4 in brain sections. With regard to why CD59 is not fully protective against AQP4-IgG injury in the central nervous system, perhaps, as mentioned above, the unique cellular and physical milieu in brain, spinal cord and optic nerve, such as the presence of microglia and a narrow extracellular space, might amplify subthreshold AQP4-IgG-induced injury. We recently reported evidence for complement bystander injury to oligodendrocytes, which lack CD59, following exposure of nearby astrocytes to AQP4-IgG and complement [
28]. While bystander cytotoxicity may be a major mechanism of cellular injury in the central nervous system, it may be inconsequential in peripheral AQP4-expressing organs.
Lastly, we acknowledge limitations in extrapolating the conclusions here from studies done in CD59−/− rats to human NMO. Though the major anatomical structures are similar in rats and humans, there are differences in the ratios of various cell types in the central nervous system such as astrocytes and neurons, and there may be differences in expression levels of CD59 and other complement inhibitor proteins. Though there is compelling evidence for the pathogenicity of AQP4-IgG and complement, the passive-transfer model used here may not fully recapitulate the pathogenesis of seropositive NMO in humans, where additional mechanisms, perhaps cytotoxic T cells, might also contribute. Finally, the data here were from short-term follow-up after systemic AQP4-IgG administration to rats, which was necessitated by the severe pathology in AQP4-IgG-treated CD59−/− rats. Peripheral organs in humans with seropositive NMO can be exposed to AQP4-IgG continuously for many years or decades. Notwithstanding these potential limitations, our results offer a logical explanation for the general absence of NMO disease outside of the central nervous system.