Skip to main content
Journal ArticleOPEN ACCESS

In vitro eradication of citrullinated protein specific B-lymphocytes of rheumatoid arthritis patients by targeted bifunctional nanoparticles

Arthritis Research and Therapy (2016) 18(1)
DOI: 10.1186/s13075-016-0918-0
26Citations
Citations of this article
54Readers
Mendeley users who have this article in their library.

This article is free to access.

Abstract

Background: Autoreactive B cells are crucial players in the pathogenesis of rheumatoid arthritis (RA). Autoantibodies specific for citrullinated proteins (ACPA), present in the serum of approximately 60-70 % of patients, have a pathogenic role in the disease. B cell depleting therapies may result in a transient immunosuppression, increasing the risk of infections. Our aim was to develop a new therapeutic approach to selectively deplete the ACPA producing autoreactive B cells. Methods: To target B cells synthetic citrullinated peptide derived from the β chain of fibrin, β60-74Cit 60,72,74 (β60-74Cit), the predominant epitope recognized by ACPA was used. Complement dependent cytotoxicity (CDC) was induced by a modified peptide derived from gp120 of HIV-1. To trigger CDC both the targeting peptide and the complement activating peptide were covalently coupled in multiple copies to the surface of poly (DL-lactic-co-glycolic acid) nanoparticles (NPs). Ex vivo antibody synthesis was examined by ELISA and ELISpot. CDC was tested after dead cell staining by flow cytometry. Results: The β60-74Cit peptide was selectively recognized by a small subset of B cells from RA patients having high level of peptide specific serum antibody, suggesting that the peptide can target diseased B cells. The modified gp120 peptide covalently coupled to NPs induced the formation of the complement membrane attack complex, C5b-9 in human serum. We show here for the first time that bifunctional NPs coupled to multiple copies of both the targeting peptide and the complement activating effector peptide on their surface significantly reduce β60-74Cit peptide specific ex vivo ACPA production, by inducing complement dependent lysis of the citrullinated peptide specific B cells of seropositive RA patients. Conclusions: Bifunctional NPs covalently coupled to autoantigen epitope peptide and to a lytic peptide activating complement may specifically target and deplete the peptide specific autoreactive B-cells.

Figures

  • Table 1 Clinical data of rheumatoid arthritis patients used in functional assays
  • Table 2 Sequences of peptides used for the ELISA experiments and for the bifunctional nanoconstructs
  • Fig. 1 Recognition of Cit-containing peptide epitope of fibrin β chain by antibodies in sera of RA patients and healthy blood donors a, b and by isolated B cells c. a Reactivities of RA (n = 170) or healthy (n = 138) serum samples with N-terminally bitotinylated β60-74Cit vs. β60-74Arg bound to neutravidin precoated plates. ELISA ratios were calculated (OD with β60-74Cit /OD with β60-74Arg). Data were analyzed with the Mann–Whitney test, and the median OD ratio of RA samples was 1.68, interquartile range 0.95–6.33, and the median OD ratio of healthy samples was 0.91, interquartile range 0.81–1.07 (***p <0.001). b Receiver operating characteristic curve analysis, area under the curve value for β60-74Cit: 0.7661. c Binding of β60-74Cit and β60-74Arg-coated fluorescent microspheres to prestimulated B cells from β60-74Cit seropositive or seronegative RA patients and from healthy individuals (n = 3/group, ELISA ratios of the selected β60-74Cit seropositive RA patients were between 10 and 15). Bars show means ± SD, *p <0.05. OD optical density, RA rheumatoid arthritis, H healthy
  • Fig. 2 β60-74Cit peptide-specific antibody secretion of purified B cells from healthy donors and RA patients. B cells were cultured for 5 days in the presence or absence of 7.5 μg/ml CpG and 1.5 ng/ml BAFF a Antibody reactivities in the supernatants against β60-74Cit (filled symbols) and β60-74Arg (open symbols) peptides were detected by ELISA. Individual data points of unstimulated b and stimulated c samples are shown. The ELISA ratios of serum samples from the same donors were between 6 and 14. n healthy = 3, nRA = 5. The data were analyzed with the paired t test, means ± SD are shown (**p <0.01, ***p <0.001). OD optical density, RA rheumatoid arthritis
  • Fig. 3 Complement activating capacities of HIV-1 gp120 derivative peptides CNNK and CNNQ and the NP-coupled CNNQK. a Pooled normal human sera (NHS) or inactivated sera were added to peptide-coated or IgG-coated plates. The deposited complement components C3, C4, and C9 were detected by anti-human C3-HRP, and anti-human C4 and C9 followed by HRP-conjugated anti-goat IgG, respectively. b C3 deposition from NHS is compared with that of C3 or C1q depleted serum and from NHS inactivated with heat or EDTA. c Comparison of C3 deposition induced by CNNK and the modified CNNQ peptide, and by human IgG. d CNNQK and β60-74Cit peptide-coupled NPs activate the C5b-9 terminal complex formation in human serum. Statistics: a, b, d analyzed with ANOVA, c analyzed with paired t test, means ± SD are shown (*p <0.05, **p <0.01, ***p <0.001). EDTA ethylenediamine tetraacetic acid, OD optical density, PLGA poly(D,L-lactic-co-glycolic acid), RA rheumatoid arthritis
  • Fig. 4 β60-74Cit and CNNQK peptide-coated bifunctional NPs suppress ex vivo synthesis of β60-74Cit specific antibodies in the presence of active complement in human sera. a PBMCs from RA patients (n = 17, ELISA ratios for β60-74Cit between 6 and 21) and b from healthy donors (n = 5) were stimulated with the TLR7/TLR8 agonist, R848, and IL-2 for 72 hours, and then the bifunctional NPs were added to the harvested cells followed by normal human sera (NHS) or heat-inactivated NHS (iNHS) at different concentrations. The number of β60-74Cit-specific IgG-producing plasma cells was counted by ELISPot. c Individual data of RA patients at 10 % iNHS and NHS are shown. d Representative ELISpot images. Statistics: a, c analyzed with paired t test, means ± SD are shown (**p <0.01, ***p <0.001). ACPA anti-citrullinated protein antibody, PBMC peripheral blood mononuclear cell, RA rheumatoid arthritis, H healthy
  • Fig. 5 Complement-dependent lysis of β60-74Cit peptide-specific B cells induced by bifunctional PLGA NPs in the presence of NHS as measured by flow cytometry. a Upper panel: representative figure of a healthy donor, lower panel: typical result with an RA patient. The binding of fluorescein-loaded NPs was detected in channel 1, dead cells were detected after TO-PRO staining in channel 4. The β60-74Cit-positive, killed B cells are detected in the right upper quadrant of the dot plot. b Individual data of five RA patients. ELISA ratios of sera of the same RA patients were between 5 and 19. Data were analyzed with paired t test, means ± SD are shown (**p <0.01). iNHS heat-inactivated normal human sera, NHS normal human sera, PLGA poly(D,L-lactic-co-glycolic acid)

Author supplied keywords

References Powered by Scopus

2010 Rheumatoid arthritis classification criteria: An American College of Rheumatology/European League Against Rheumatism collaborative initiative

Arthritis and Rheumatism
7146Citations
N/AReaders
Get full text

Induction of osteoclastogenesis and bone loss by human autoantibodies against citrullinated vimentin

Journal of Clinical Investigation
623Citations
N/AReaders
Get full text

The epidemiology of rheumatoid arthritis

Rheumatic Disease Clinics of North America
600Citations
N/AReaders
Get full text
View more at Scopus

Cited by Powered by Scopus

The inositol trisphosphate/calcium signaling pathway in health and disease

Physiological Reviews
544Citations
N/AReaders
Get full text

Rheumatoid arthritis microenvironment insights into treatment effect of nanomaterials

Nano Today
102Citations
N/AReaders
Get full text

The interaction between nanoparticles and immune system: application in the treatment of inflammatory diseases

Journal of Nanobiotechnology
93Citations
N/AReaders
Get full text
View more at Scopus

Register to see more suggestions

Mendeley helps you to discover research relevant for your work.

Already have an account?

Cite

CITATION STYLE

APA

Pozsgay, J., Babos, F., Uray, K., Magyar, A., Gyulai, G., Kiss, É., … Sármay, G. (2016). In vitro eradication of citrullinated protein specific B-lymphocytes of rheumatoid arthritis patients by targeted bifunctional nanoparticles. Arthritis Research and Therapy, 18(1). https://doi.org/10.1186/s13075-016-0918-0

Readers over time

‘16‘17‘18‘19‘20‘21‘22‘23‘24‘250481216

Readers' Seniority

Tooltip

PhD / Post grad / Masters / Doc 24

75%

Researcher 4

13%

Professor / Associate Prof. 3

9%

Lecturer / Post doc 1

3%

Readers' Discipline

Tooltip

Immunology and Microbiology 8

31%

Chemistry 7

27%

Medicine and Dentistry 6

23%

Agricultural and Biological Sciences 5

19%

Save time finding and organizing research with Mendeley

Sign up for free
0