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South African Journal of Science

On-line version ISSN 1996-7489
Print version ISSN 0038-2353

S. Afr. j. sci. vol.113 n.7-8 Pretoria Jul./Aug. 2017

http://dx.doi.org/10.17159/sajs.2017/20160244 

RESEARCH ARTICLE

 

Conservation implications of avian malaria exposure for African penguins during rehabilitation

 

 

Annelise BotesI; Hanlie ThiartI; Nola J. ParsonsII, III; Dirk U. BellstedtI

IDepartment of Biochemistry, Stellenbosch University, Stellenbosch, South Africa
IISouthern African Foundation for the Conservation of Coastal Birds, Cape Town, South Africa
IIIBayworld Centre for Research and Education, Port Elizabeth, South Africa

Correspondence

 

 


ABSTRACT

The African penguin (Spheniscus demersus) is the only penguin species that breeds on the African continent and it is currently classified as endangered. Its conservation is assisted by the Southern African Foundation for the Conservation of Coastal Birds (SANCCOB) which is a seabird rehabilitation facility based at the Rietvlei Wetland Reserve in Tableview, Cape Town. Despite the success of SANCCOB in rehabilitating diseased, injured or oiled penguins, significant mortalities have occurred at the facility as a result of avian malaria. Avian malaria can be contracted during rehabilitation during which penguins are inadvertently exposed to additional threats. An enzyme-linked immunosorbent assay (ELISA) was used to assess the anti-Plasmodium antibody levels of penguins to avian malaria on entry into the SANCCOB facility from 2001 to 2004 and during their rehabilitation process. Using blood smear data, avian malaria prevalence and malaria-related deaths were also monitored from 2002 to 2013. Significant increases in anti-Plasmodium antibody levels after admission were found during summer months. New infection and not parasite recrudescence was concluded to be the cause of this increase. This source was confirmed by a dramatic drop in penguin mortalities upon exclusion of mosquito vectors in 2008. Mortalities did not depend on the birds' abilities to produce an anti-Plasmodium antibody response and oiling had no influence on immunity or prevalence of avian malaria infections. This study highlights the importance of mosquito vector control to control pathogen exposure in wild bird rehabilitation centres.
SIGNIFICANCE:
Efforts to assist with the conservation of endangered species can unintentionally add to the conservation burden.
Rehabilitation influences exposure of African penguins to avian malaria.
Avian malaria prevalence and mortality are not influenced by oiling or anti-Plasmodium antibody responses.
Vector control can limit avian malaria exposure in wild bird rehabilitation centres.

Keywords: Plasmodium; antibody response; ELISA; SANCCOB; vector control


 

 

Introduction

The African penguin (Spheniscus demersus) is the only penguin species that breeds on the African continent. Their numbers have decreased from an estimated 1.5-3 million before 1900 to fewer than 26 000 breeding pairs in 20091,2 - a decline which has resulted in their conservation status being changed from vulnerable to endangered2. Since the late 1800s, a sequence of threats has led to their decline. Breeding habitats were reduced through guano collection, followed by egg collection for human consumption, overexploitation of prey species and, recently, oiling events caused by oil spills.1 Furthermore, blood parasites such as Plasmodium, which causes avian malaria, are ongoing threats leading to further mortalities.3,4

The Southern African Foundation for the Conservation of Coastal Birds (SANCCOB) maintains a seabird rehabilitation facility based at the Rietvlei Wetland Reserve in Tableview, Cape Town. They rehabilitate diseased, injured or oiled seabirds, of which most are African penguins. Through SANCCOB's efforts, African penguins have been able to survive in the wild after release and have successfully returned to breeding.5 Unfortunately, avian malaria infections and associated mortalities in African penguins do occur at the facility.3,4

Internationally, avian malaria is a known cause of mortality in captive penguins kept in outdoor displays or zoos with P. relictum and P. elongatum being the associated parasites.6-10 In the case of wild birds, P. tejerai, P. cathemerium, P. nucleophilum and P. unalis could be identified in Magellanic penguins (S. magellanicus) undergoing rehabilitation along the coast of Brazil.11 The first report of a Plasmodium infection in an African penguin in the wild was from Saldanha Bay, described as P. relictum subsp. spheniscidae.12 Brossy et al.4 identified P. relictum in wild African penguins being rehabilitated at SANCCOB, but rarely found parasitaemia in penguins at their breeding colonies. These findings were based on blood smear analysis; when using anti-Plasmodium antibody levels as an indicator of avian malaria exposure, both wild and captive African penguins were found to be exposed to avian malaria.4,13 In addition, about 30% of penguins admitted to SANCCOB were already malaria positive based on blood smear analysis, on entry into the facility, indicating exposure of the wild population to the pathogen.3 It was subsequently suggested that wild and captive penguins were being exposed to different Plasmodium species4 which could explain the higher levels of infection and mortality experienced during rehabilitation.3,13 In captivity, there is an increased chance of being exposed to mosquito vectors that could act as a reservoir for land bird avian malaria parasites.14,15

The impact of avian malaria on the decline of wild avian populations is best illustrated by the history of native Hawaiian bird species. Examples are the the Hawaiian crow, or Alalã (Corvus hawaiiensis), which is now extinct in the wild16, and the Hawaiian honeycreepers (Drepanidinae) of which most species are either extinct or critically endangered17. In the case of the Galápagos penguin (S. mendiculus), the introduction of Plasmodium to the Galápagos Islands is causing concern about the effect this introduction will have on the survival of this endangered species.18 Because seabirds breed in relatively small geographical areas, they are sensitive to environmental changes, with population declines as a possible consequence.19 Population declines in turn increase the vulnerability to diseases.20 As a result, there is a need for dedicated rescue and rehabilitation centres that play a significant role in ensuring the conservation of species, but they could inadvertently be exposing animals to new threats.21 The possibility of introducing a foreign avian malaria parasite into African penguins during rehabilitation is therefore a major concern, as subsequent introduction into wild breeding populations could cause a further decline in an already endangered seabird population.

During rehabilitation at SANCCOB, efficient treatment of avian malaria requires early diagnosis, because it is often too late for treatment once clinical signs appear. Screening for blood parasites is therefore conducted through routine blood smear evaluation, but serious pathological effects and even death can occur prior to the appearance of parasites in circulating erythrocytes.22 The lack of parasites in erythrocytes also does not exclude their possible presence in the endothelium or haemopoietic tissue.6,7,23 Furthermore, Babesia infections cannot easily be distinguished from Plasmodium infections by blood smear.24 The polymerase chain reaction (PCR) can be used as an alternative diagnostic technique as it is viewed to be more sensitive and highly specific and does not rely on visualisation of the parasite.25 Unfortunately, similarly to blood smears, the method relies on the presence of circulating blood parasites26 and therefore these methods are not always a true reflection of parasite exposure13,26.

On the basis of cross-reactivity between anti-Plasmodium antibodies, Graczyk et al.23 developed an enzyme-linked immunosorbent assay (ELISA) for the detection of anti-P. relictum and anti-P. elongatum antibodies. It was found to be an effective tool for diagnosing exposure to avian malaria in penguins.27 The ELISA made use of a recombinant polypeptide (R32tet32) as capture antigen, which consisted of 32 tetrapeptides - 31 with the sequence NANP and 1 with the sequence NVDP followed by a 32 amino acid hydrophobic tail.28 The sequence was derived from the highly immunogenic repeat region of the circumsporozoite (CS) protein of P. falciparum. CS-proteins are uniformly distributed over the entire membrane surface of sporozoites, which is the first stage of the parasite in the avian host after being infected. Immunological cross-reactivity is known to exist against the CS-proteins of unrelated species and this may be as a result of structural and functional similarities of the secondary and tertiary structures resulting in common epitopes.23,29-31

The objectives of this study were, firstly, to evaluate the exposure of wild African penguins to avian malaria during rehabilitation at SANCCOB by measuring anti-Plasmodium antibody levels using an ELISA similar to that of Graczyk et al.23; secondly, to determine the influence of these antibody levels on survival during rehabilitation and the effect of oiling on antibody levels and, finally, to show the effect of vector exclusion on the incidence of malaria-related deaths at SANCCOB.

 

Materials and methods

Sample collection and processing

Anti-Plasmodium antibody levels of African penguins upon entry to the SANCCOB facility, and for up to 3 weeks after admission, were assessed in birds admitted from October 2001 to January 2004. Penguins were admitted for various reasons such as oiling, poor condition, injury, abandonment or arrested moulting. No specific age group was targeted.

As part of SANCCOB's health monitoring procedures,3 weekly blood samples were routinely taken from all penguins present in the rehabilitation facility for blood smear analysis. Sampling of blood entailed insertion of a 23-gauge needle into the intradigital foot vein of a penguin and collection into a heparinised capillary tube. Thin blood smears were prepared immediately after blood collection and slides were fixed with methanol and stained with a modified Wright-Giemsa stain (Kyron Laboratories, Johannesburg, South Africa). For antibody analysis, a single 50 mL blood volume, as measured by calibrated heparinised capillary tubes, was deposited on filter paper (Immunovet Services, Johannesburg, South Africa) and air dried.27 Prior to ELISA testing, blood was eluted overnight at 4 °C from each of the filter papers with 333.33 mL Millipore water containing 0.4% Tween 20.23

Birds were rehabilitated and released as soon as deemed fit to survive in the wild.3 Consequently, there was a difference in the number of data points collected for each bird. The aim was to obtain at least 30 samples per week and therefore released birds were replaced with newly admitted birds, unless fewer birds were actually being rehabilitated, at any given time.

Positive and low or negative control sera were obtained from the routine blood samples. The positive control was from a penguin that tested malaria positive on blood smear and had a high anti-Plasmodium antibody titre in our ELISA. The negative control was from a penguin chick that was artificially hatched and raised in a vector-free environment before being admitted to SANCCOB for rehabilitation.

ELISA capture antigen

Ballou et al.32 synthesised peptides containing 8-16 residues of the CS-protein repeat region of P. falciparum containing the sequence NANP. Antibodies against these peptides were able to recognise native CS-protein and therefore a peptide with the sequence (NANP)4 was used as capture antigen in this study. To allow for conjugation to bovine serum albumin (BSA) the peptide was synthesised containing a S-acetylmercaptosuccinic anhydride (SAMSA) group coupled to its N-terminal side. Synthesising the SAMSA-peptide (Biopep Laboratories, Stellenbosch University, Stellenbosch, South Africa) allowed the preparation of a capture antigen free of contaminating serum proteins that could cause cross-reactions in the ELISA. The purity of the peptide was confirmed by electrospray mass spectrometry analysis.

Prior to use, the peptide was conjugated to BSA in a 3:1 ratio to allow for a more rigid attachment of the peptide to the polystyrene surface of the microtitre plate.33 This step prevents desorption of antigen during ELISA incubation and wash steps. Conjugation consisted of three reaction steps: the introduction of maleimide groups into BSA, introduction of a sulfhydryl group into the malaria peptide and conjugation of the malaria peptide to the activated BSA.34-38 To ensure that the peptide-BSA conjugate solution was not contaminated with smaller or larger complexes, it was subjected to gel filtration chromatography using a G-25 Sephadex column.

Penguin anti-Plasmodium antibody ELISA

Microtitre plates (96 well, MediSorpTM, Thermo ScientificTM, NuncTM, Roskilde, Denmark) were coated overnight at 4 °C with 0.5 mg/mL (100 mL/well) of the 3:1 peptide-BSA conjugate in carbonate buffer (50 mM, pH 9.6). The coating solution was decanted and the plate blocked (1 h, 37 °C) with casein buffer (0.5% casein, 0.15 M NaCl, 0.01 M Tris-HCl, 0.02% thiomersal, pH 7.6, 200 mL/well). Filter paper eluates were diluted 1/50 and serum 1/200 in casein buffer containing 0.1% Tween 20 (casein-Tween), added to wells in triplicate (100 mL/well) and incubated (3 h, 37 °C). Biotinylated rabbit anti-penguin Ig antibody was prepared as described33 and added (100 mL/well) after being diluted 1/100 in casein-Tween. After incubation (1 h, 37 °C), avidin-horseradish-peroxidase conjugate (Zymed®, San Francisco, CA, USA) diluted 1/100 in casein-Tween was added (100 mL/well) and the plates were further incubated (1 h, 37 °C). Finally, the substrate solution (ABTS, 0.015% H2O2 in 0.1 M citrate buffer, pH 5, 100 mL/well) was added and the absorbance measured after 30 min at 37 °C on a Labsystems Multiskan MS spectrophotometer at 405 nm. Between all steps, the plates were washed three times, except after coating, with phosphate-buffered saline (PBS; 200 mL/well) containing 0.1% Tween 20,. Negative and positive control sera were included on each plate to monitor inter-assay variation. The ability of the capture antigen to distinguish between malaria positive and negative sera as well as non-specific reactions towards activated BSA were also evaluated.

Data analysis

ELISA data from October 2001 to January 2004 were grouped together into 2-month periods. Because penguins were being admitted continuously within a specific 2-month period, the week of entry for all penguins in that period was taken as Week 0 and subsequent weeks of sampling as Weeks 1 and 2.

The absorbance values measured during ELISA analysis are referred to as ELISA titres which represent anti-Plasmodium antibody levels. The change in antibody levels, one and two weeks after admission, were calculated for each 2-month period. This calculation was done by subtracting the average titre value obtained at Week 0 from that obtained at Week 1 and again at Week 2. The resulting two values were plotted graphically for each 2-month period.

Most penguins were rehabilitated for no longer than 2-3 weeks after admission and therefore only the data for Weeks 0, 1 and 2 were used for statistical analysis using the general linear models procedure in the Statistical Analysis System (SAS) Enterprise Guide (version 1.3.0.161). Weather data were obtained from Weather Underground and Harris et al.39

Monitoring the prevalence of avian malaria

The prevalence of avian malaria (number of samples positive during rehabilitation divided by the number of individual bleeds) was also determined for the facility as a whole. This determination was based on blood smear analysis which is routinely performed and therefore allowed for long-term monitoring (2002-2013). Plasmodium diagnosis was based on identification of trophozoites and gametocytes in the erythrocytes with the latter used to distinguish from Babesia infections. Meronts were rarely identified. Deaths that occurred as a result of avian malaria were confirmed during post-mortem examinations as described.40

 

Results

Penguin anti-Plasmodium antibody ELISA

Gel filtration chromatography produced a single peak indicating that the conjugate consisted of a single complex (Supplementary figure 1). ELISA titres of positive and negative penguin serum samples indicated that anti-Plasmodium antibodies were able to cross-react with the peptide-BSA conjugate (Supplementary figure 2) and this interaction was primarily aimed at the peptide.

Anti-Plasmodium antibody response

The increase in anti-Plasmodium antibody levels after admission to the SANCCOB facility is shown in Figure 1. In penguins admitted from October to November 2001, an increase in antibody levels could only be observed by Week 2. In penguins admitted from December 2001 to January 2002, there was an earlier increase in antibody levels one week after entering the facility and this pattern continued for penguins admitted during the warmer months until March 2002. This period coincided with an increase in the number of birds that tested positive for malaria by blood smear during rehabilitation (Table 1). As ambient temperatures started to drop, so did the increase in antibody responses one week after admission as well as the percentage of penguins that tested blood smear positive (BS+). Antibody levels started to increase again after admission during October-November 2002, but at much lower levels than those during 2001. A more pronounced increase in antibody levels, however, followed during February-May 2003 compared to the same period in 2002, but this increase did not coincide with an increase in BS+ penguins (Table 1). The elevation in antibody levels in 2003 again decreased as temperatures dropped (June-July), and then increased slightly as temperatures started to increase (August-September), but BS+ cases during rehabilitation only started to increase after the August-September 2003 period. Analysis indicated a significant association between the average increase in ELISA titre values 2 weeks after admission and average day (p=0.028) and night (p=0.008) temperatures (see the supplementary material).

Influence of anti-Plasmodium antibody response on survival

The increase in anti-Plasmodium antibody levels in penguins that were released and those that died during rehabilitation are shown in Figure 2. Although these data indicated that the penguins were responding to Plasmodium infections by producing an antibody response, the difference in response between the released and deceased penguins was not statistically significant.

Malaria blood smear data for the penguins that were released vs those that died for each of the respective 2-month periods are shown in Table 1 along with the percentage of deaths as a result of malaria as confirmed by post-mortem examination. All penguins that died during rehabilitation as a result of malaria were also those that tested BS+ for malaria resulting in the percentage BS+ cases and malaria deaths being the same. The only exception was the birds sampled in February-March 2003, for which not all deaths were as a result of malaria - only 20% were malaria-related deaths.

Influence of oiling on the anti-Plasmodium antibody response

The effect of oiling on the increase in anti-Plasmodium antibody levels is shown in Figure 3. No statistically significant difference was found between oiled and not oiled penguins except for the period December 2001 to January 2002. The significant difference (p=0.0136) is, however, questionable as there were only four oiled penguins during this period and the difference was caused by the high titre of a single penguin that was oiled and that died during rehabilitation.

Malaria blood smear results of the oiled versus not oiled penguins during rehabilitation and the number of penguins that died as a result of malaria are shown in Table 2. The number of birds that tested positive for malaria by blood smear and that died as a result of malaria during rehabilitation were on average higher in the not oiled group.

Monitoring the prevalence of avian malaria

The prevalence of avian malaria and the deaths specifically related to avian malaria at SANCCOB in the period from 2002 to 2013 are shown in Table 3. These data show a persistent level of avian malaria infection in penguins being rehabilitated during the period from 2001 to 2008. There is, however, not always a good correlation between avian malaria prevalence and malaria-specific deaths, which indicates the inefficiency of blood smear analysis as a diagnostic tool. A mosquito-proof net was installed over the open-air part of the facility in October 2008, after which there was a sharp decrease in the prevalence of and deaths as a result of avian malaria.

 

Discussion

In previous studies, penguins were reported to harbour Plasmodium (in the erythrocytic stages of infection) upon admission,3 which implied that they had already been infected in the wild. In this study, Plasmodium could be detected in some penguins during rehabilitation when using blood smear analysis, which may indicate prior exposure in the wild. As observed in other studies, the BS+ cases increased in the warmer months and decreased in the colder months3, which can be attributed to the negative influence of cooler temperatures on the distribution of mosquito vectors, with a subsequent decrease in malaria infections22,41. Prior exposure to Plasmodium does not preclude the possibility of penguins being confronted with a different Plasmodium species in captivity4, given that co-infections are possible42 and that as expected25,26, the changes in anti-Plasmodium antibody levels did not always coincide with increases in malaria BS+ cases.

If penguins survive their first infection of avian malaria, their immune system appears to be capable of reducing the number of parasites with a resulting low-level infection (premunition) resulting from survival of latent parasites.43 This premunition allows penguins to control a new infection with a rapid and intensified antibody response. Recrudescence, which is an increase in the number of latent parasites in the blood and therefore the development of symptoms, can be induced in birds with premunition by stress factors such as nutritional, environmental or migration stress.7 The rehabilitation process itself stresses penguins, which could lead to recrudescence in penguins that enter the SANCCOB facility with an existing low-level infection.4 However, if existing infections, and therefore recrudescence, were the main cause of antibody responses seen in penguins being rehabilitated, then the same increase in antibody levels should be seen throughout the year, irrespective of season. An increase in the anti-Plasmodium antibody response was, however, only observed during the warmer spring and summer months (October-March); a reduced response was observed during the colder autumn and winter months (April-September). The pattern of antibody increase and decrease did, however, shift from one year to the next because of differences in weather patterns between years. The climate along the South African west and south coasts exhibits variable temperatures and rainfall conditions (Supplementary table 1) that in turn can influence vector and parasite abundance and host exposure.44 November 2002 experienced a higher than normal rainfall which could have caused a hatch delay with an increase in mosquito populations in subsequent months,45 causing a larger increase in anti-Plasmodium antibodies measured during February-May 2003 as well as an increase in malaria-specific deaths in 2003 compared to 2002 (Table 3).

In an attempt to reduce malaria infections in the facility, mosquito-proof netting was installed at the facility in 2008. A significant decrease in the prevalence of avian malaria after the installation provided conclusive evidence that avian malaria infections in the SANCCOB facility were primarily a result of new infections and not recrudescence. However, the very low numbers of penguins that contracted avian malaria in the facility after 2008 can probably be ascribed to existing infections upon admission and therefore parasite recrudescence.

New infections rely on the presence of a vector as well as a suitable avian reservoir host. It is therefore unlikely that natural infections in penguins will occur in the absence of infected wild birds.14 If African penguins are naturally infected with P. relictum or a subspecies thereof12,24 and have developed resistance against this species, it might be that they are exposed to possible infection by other malaria species during rehabilitation. The SANCCOB rehabilitation facility is adjacent to a large shallow freshwater lake (Rietvlei) with abundant bird life as well as large numbers of culicine mosquitoes. This scenario could facilitate host switching with resulting Plasmodium infections to which penguins are not exposed in their natural environment.46Plasmodium spp. are known for their low specificity and broad host range which allows for host switching between different mosquito vectors as well as avian hosts.47 Host switching could also cause a parasite to undergo a change in virulence48 which could translate into an acute infection. Even if penguins survive these new infections during rehabilitation, they could become carriers and introduce this Plasmodium species into breeding colonies, thereby exposing the population to a new hitherto unknown Plasmodium. In future studies, it would be worthwhile to confirm, using molecular methods,49 the identity of the Plasmodium species that infect penguins during rehabilitation in comparison to those infecting breeding colonies, as well as relevant reservoir hosts.

If penguins are infected during rehabilitation, their survival may be influenced by their physical condition upon admission and thus their ability to produce an anti-Plasmodium antibody response. If the response is too low or delayed, the bird is likely to succumb.43 We found no difference in the antibody reponses between penguins that survived and were released after rehabilitation versus those that died as a result of malaria during rehabilitation. Survival therefore did not depend on antibody response alone. The mortality results can, however, be viewed as being biased because all penguins diagnosed as malaria BS+ were treated against malaria.

Apart from large oiling events, penguins are admitted to SANCCOB as a result of chronic oiling throughout the year.3,50 Oiling is one of the major human threats to penguin conservation worldwide. Oiling causes the feathers to lose their natural insulative and waterproofing properties and ingested oil can lead to internal organ damage as well as anaemia and a depression of immune function.50,51 An altered immune function could make them more susceptible to malaria infection during rehabilitation. In this study, oiling was found not to influence the ability of penguins to produce an anti-Plasmodium antibody response. A possible explanation for this finding may be that, because of the presence of conservation staff monitoring most of the African penguin breeding colonies and public awareness, penguins are brought to SANCCOB soon after oiling, and are generally strong on arrival.3 Furthermore, not oiled penguins were admitted throughout the year whilst the majority of oiled penguins were seen in winter months when there are fewer malaria infections, as diagnosed by blood smear, as well as fewer malaria-specific deaths. From this observation it can be concluded that oiling had no effect on the prevalence of malaria in African penguins that were being rehabilitated.

 

Conclusion

This research highlights the importance of mosquito vector control in order to control avian malaria in wild bird rehabilitation centres. Blood smear results indicated that birds are being exposed to avian malaria in the wild, but anti-Plasmodium antibody responses indicated that penguins were in all likelihood being newly infected by mosquitoes during rehabilitation. This was further confirmed by a sharp decline in malaria prevalence after vector control measures were implemented at SANCCOB in the form of mosquito netting. Further studies are needed to confirm whether penguins are confronted with a different Plasmodium species during rehabilitation than in the wild. Also, determining the source of infections will allow effective management of the disease by establishing conservation strategies to either control or prevent future infections during rehabilitation.

 

Acknowledgements

We thank the staff and volunteers from SANCCOB for facilitating this research. SANCCOB is supported by a wide range of donors, including the International Fund for Animal Welfare, Hans Hoheisen Charitable Trust and the National Lottery Distribution Trust Fund. N.J.P. is supported by the Sea Research Foundation (Mystic Aquarium), the Georgia Aquarium and the Leiden Conservation Foundation. This research was funded by the World Wildlife Fund (project number ZA 5020).

 

Authors' contributions

A.B. was responsible for methodology development, antibody analysis, curation of ELISA data, data collection, writing the initial draft and manuscript revision. H.T. was responsible for antibody analysis, curation of ELISA data and data collection. N.J.P. was responsible for blood and serum collection, data collection, curation of blood smear and malaria data, and manuscript revision. D.U.B. was responsible for conceptualisation of the project, acquisition of funding, methodology development and manuscript revision.

 

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Correspondence:
Annelise Botes
Email: annelise@sun.ac.za

Received: 14 Aug. 2016
Revised: 20 Dec. 2016
Accepted: 15 Feb. 2017

 

 

FUNDING: World Wildlife Fund (South Africa)

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