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AMERICAN COLLEGE OF RHEUMATOLOGY

                                             POSITION STATEMENT

     SUBJECT:                            Methodology of Testing for Antinuclear Antibodies

     PRESENTED BY:                        American College of Rheumatology

     FOR DISTRIBUTION TO:                Members of the American College of Rheumatology
                                         Medical Societies
                                         Managed Care Organizations/Third Party Carriers
                                         Laboratories

     SUMMARY:

 1       •    The immunofluorescence antinuclear antibody (ANA) assay is the gold standard for ANA testing
 2            with greater sensitivity than solid phase assays.
 3
 4       •    HEp-2 cells have approximately 100 to 150 possible autoantigens. These cells are used to detect
 5            ANAs by the immunofluorescence (IF) method, in which both pattern and titer can be described,
 6            and to display a variety of autoantigens not present in multiplex ANA tests.
 7
 8       •    Many commercial laboratories and some hospital laboratories have switched their ANA screening
 9            test to solid phase immunoassays, such as a multiplex platform. The latter technique can screen
10            and process large volumes of clinical specimens more quickly and at less cost than the traditional
11            immunofluorescence ANA test using fixed HEp-2 cells as substrate.
12
13       •    These multiplex assays can detect only the specific autoantibodies directed against the limited
14            number (typically 8-10) autoantigens that are displayed.
15
16       •    Laboratories should indicate the method used when reporting ANA results.
17
18   BACKGROUND:
19
20   The methodology of the tests for the detection of antinuclear antibodies has changed over the years from
21   the LE cell prep, to immunofluorescence utilizing sections of various rodent organs (e.g. rat or mouse liver
22   or kidney, etc.) to cell lines, in particular HEp-2. HEp-2 cells contain approximately 100 to 150
23   autoantigens. These cells are used to detect ANA by the immunofluorescence method, in which both
24   pattern and titer can be described, and to display a variety of autoantigens not present in the multiplex ANA
25   tests. Researchers have seen the evolution of methodology of tests for the detection of particular ANAs
26   (anti-DNA, Sm, RNP, Ro/SS-A, La/SS-B, etc.) from immunodiffusion, complement-fixation,
27   hemagglutination, to various solid phase immunoassays.
28
29   Over the years, numerous investigators and commercial organizations have attempted to develop solid
30   phase immunoassays for the detection of ANA and specific ANAs, which are easier and cheaper to perform
31   and standardize compared to immunofluorescence assays using fixed HEp-2 cells as a substrate. A review
32   of the literature by the committee indicates that up to 35% of patients with SLE and a positive ANA by
33   immunofluorescence (IF) were negative on solid phase assays (1-4, 6-21, 23). Many commercial laboratories
34   and some hospital laboratories have switched their antinuclear antibody (ANA) screening test to solid
35   phase immunoassays, such as a multiplex platform, for the reasons noted above, and since the latter
36   technique can screen and process large volumes of clinical specimens than the traditional
37   immunofluorescence ANA test using fixed HEp-2 cells as substrate.
38
39   Various national and international organizations have also been involved in the standardization of these
40   tests for the harmonization of laboratory results. These include World Health Organization, Centers for
41   Disease Control, Dutch Red Cross and the International Union of Immunological Societies (5).
42
43   Any laboratory test, to be most useful, must maximally distinguish patients with a particular disorder from
44   related disorders. It is understood that both commercial and hospital laboratories are interested and
45   committed to providing the best laboratory tests for the diagnosis of rheumatic diseases.
46
47   The immunofluorescence ANA test is the gold standard for ANA testing. When performed with a history
48   and physical, it identifies almost all patients with systemic lupus erythematosus (sensitivity over 95%)(22),
49   although the specificity of this assay is only 57% for SLE when compared to patients with related
50   rheumatic and autoimmune disorders(22). In addition, the IF ANA is an important test for the screening and
51   diagnosis of systemic sclerosis (sensitivity 85%), polymyositis/dermatomyositis (sensitivity 61%), primary
52   Sjogren’s syndrome (sensitivity 48%), juvenile idiopathic arthritis (sensitivity 57%), drug-induced lupus
53   (sensitivity 100%), mixed connective tissue disease (sensitivity 100%), and autoimmune hepatitis as well as
54   being important in monitoring and assessing prognosis in individuals with Raynaud’s phenomenon.
55
56
57   RECOMMENDATIONS:
58
59       •    The immunofluorescence (IF) ANA test should remain the gold standard for ANA testing.
60
61       •    Hospital and commercial laboratories using bead-based multiplex platforms or other solid phase
62            assays for detecting ANAs must provide data to ordering physicians on request that their assay has
63            the same or improved sensitivity and specificity compared to the IF ANA.
64
65       •    In-house assays for detecting ANA as well as anti-DNA, anti-Sm, anti-RNP, anti-Ro/SS-A, anti-
66            La/SS-B, etc. should be standardized according to national (e.g., CDC) and/or international (e.g.,
67            WHO, IUIS) standards.
68
69       •    Laboratories should specify the methods utilized for detecting ANAs when reporting their results.
70
71   REFERENCES:
72
73       1.   Avaniss-Aghajani, E., Berzon, S., and Sarkissian, A. 2007. Clinical value of multiplexed bead-
74            based immunoassays for detection of autoantibodies to nuclear antigens. Clin Vaccine Immunol
75            14:505-509.
76       2.   Bernardini, S., Infantino, M., Bellincampi, L., Nuccetelli, M., Afeltra, A., Lori, R., Biroccio, A.,
77            Urbani, A., and Federici, G. 2004. Screening of antinuclear antibodies: comparison between
78            enzyme immunoassay based on nuclear homogenates, purified or recombinant antigens and
79            immunofluorescence assay. Clin Chem Lab Med 42:1155-1160.
80       3.   Biagini, R.E., Parks, C.G., Smith, J.P., Sammons, D.L., and Robertson, S.A. 2007. Analytical
81            performance of the AtheNA MultiLyte ANA II assay in sera from lupus patients with multiple
82            positive ANAs. Anal Bioanal Chem 388:613-618.
83       4.   Bonilla, E., Francis, L., Allam, F., Ogrinc, M., Neupane, H., Phillips, P.E., and Perl, A. 2007.
84            Immunofluorescence microscopy is superior to fluorescent beads for detection of antinuclear
85            antibody reactivity in systemic lupus erythematosus patients. Clin Immunol 124:18-21.
86       5.   Bossuyt et al Ann Rheum Dis 2008; 67:1061-1063
87       6.   Caramaschi, P., Ruzzenente, O., Pieropan, S., Volpe, A., Carletto, A., Bambara, L.M., and Biasi,
88            D. 2007. Determination of ANA specificity using multiplexed fluorescent microsphere
89            immunoassay in patients with ANA positivity at high titres after infliximab treatment: preliminary
90            results. Rheumatol Int 27:649-654.
91       7.   Case Records of the Mass General Hospital. Case 5-2009: A 47-year-old woman with a rash and
92            numbness and pain in the legs. New Engl J Med 2009; 360:7---720.
93       8.   Copple, S.S., Martins, T.B., Masterson, C., Joly, E., and Hill, H.R. 2007. Comparison of three
94            multiplex immunoassays for detection of antibodies to extractable nuclear antibodies using
95            clinically defined sera. Ann N Y Acad Sci 1109:464-472.
96      9.    Eissfeller, P., Sticherling, M., Scholz, D., Hennig, K., Luttich, T., Motz, M., and Kromminga, A.
 97            2005. Comparison of different test systems for simultaneous autoantibody detection in connective
 98            tissue diseases. Ann N Y Acad Sci 1050:327-339.
 99      10.   Ghillani, P., Rouquette, A.M., Desgruelles, C., Hauguel, N., Le Pendeven, C., Piette, J.C., and
100            Musset, L. 2007. Evaluation of the LIAISON ANA screen assay for antinuclear antibody testing in
101            autoimmune diseases. Ann N Y Acad Sci 1109:407-413.
102      11.   Gniewek RA, Stites DP, McHugh TM, Hilton JF, Nakagawa M. Comparison of antinuclear
103            antibody testing methods: immunofluorescence assay versus enzyme immunoassay. Clin Diagn
104            Lab Immunol. 1997 Mar;4(2):185-8.
105      12.   Gonzalez, C., Garcia-Berrocal, B., Perez, M., Navajo, J.A., Herraez, O., and Gonzalez-Buitrago,
106            J.M. 2005. Laboratory screening of connective tissue diseases by a new automated ENA screening
107            assay (EliA Symphony) in clinically defined patients. Clin Chim Acta 359:109-114.
108      13.   Homburger HA, Cahen YD, Griffiths J, Jacob GL. Detection of antinuclear antibodies:
109            comparative evaluation of enzyme immunoassay and indirect immunofluorescence methods.Arch
110            Pathol Lab Med. 1998 Nov;122(11):993-9.
111      14.   Lopez-Hoyos, M., Rodriguez-Valverde, V., and Martinez-Taboada, V. 2007. Performance of
112            antinuclear antibody connective tissue disease screen. Ann N Y Acad Sci 1109:322-329.
113      15.   Martins, T.B., Burlingame, R., von Muhlen, C.A., Jaskowski, T.D., Litwin, C.M., and Hill, H.R.
114            2004. Evaluation of multiplexed fluorescent microsphere immunoassay for detection of
115            autoantibodies to nuclear antigens. Clin Diagn Lab Immunol 11:1054-1059.
116      16.   Nifli, A.P., Notas, G., Mamoulaki, M., Niniraki, M., Ampartzaki, V., Theodoropoulos, P.A.,
117            Kopnitsky, M.J., and Castanas, E. 2006. Comparison of a multiplex, bead-based fluorescent assay
118            and immunofluorescence methods for the detection of ANA and ANCA autoantibodies in human
119            serum. J Immunol Methods 311:189-197.
120      17.   Nossent, H., and Rekvig, O.P. 2001. Antinuclear antibody screening in this new millennium:
121            farewell to the microscope? Scand J Rheumatol 30:123-126; discussion 127-128.
122      18.   Olaussen, E., and Rekvig, O.P. 1999. Screening tests for antinuclear antibodies (ANA): selective
123            use of central nuclear antigens as a rational basis for screening by ELISA. J Autoimmun 13:95-
124            102.
125      19.   Shovman, O., Gilburd, B., Zandman-Goddard, G., Yehiely, A., Langevitz, P., and Shoenfeld, Y.
126            2005. Multiplexed AtheNA multi-lyte immunoassay for ANA screening in autoimmune diseases.
127            Autoimmunity 38:105-109.
128      20.   Sinclair, D., Saas, M., Williams, D., Hart, M., and Goswami, R. 2007. Can an ELISA replace
129            immunofluorescence for the detection of anti-nuclear antibodies?--The routine use of anti-nuclear
130            antibody screening ELISAs. Clin Lab 53:183-191.
131      21.   Smith, J., Onley, D., Garey, C., Crowther, S., Cahir, N., Johanson, A., Painter, S., Harradence, G.,
132            Davis, R., and Swarbrick, P. 2005. Determination of ANA specificity using the UltraPlex
133            platform. Ann N Y Acad Sci 1050:286-294.
134      22.   Solomon et al. Evidence-based guidelines for the use of immunologic testing: ANA. Arth Care
135            Res 2002;47:434-444.
136      23.   Ulvestad, E. 2001. Performance characteristics and clinical utility of a hybrid ELISA for detection
137            of ANA. Apmis 109:217-222.
138
139
140   Approved by the Committee on Rheumatologic Care: 01/2009
141   Approved by the Board of Directors: 02/2009

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ANA Position Statement

  • 1. AMERICAN COLLEGE OF RHEUMATOLOGY POSITION STATEMENT SUBJECT: Methodology of Testing for Antinuclear Antibodies PRESENTED BY: American College of Rheumatology FOR DISTRIBUTION TO: Members of the American College of Rheumatology Medical Societies Managed Care Organizations/Third Party Carriers Laboratories SUMMARY: 1 • The immunofluorescence antinuclear antibody (ANA) assay is the gold standard for ANA testing 2 with greater sensitivity than solid phase assays. 3 4 • HEp-2 cells have approximately 100 to 150 possible autoantigens. These cells are used to detect 5 ANAs by the immunofluorescence (IF) method, in which both pattern and titer can be described, 6 and to display a variety of autoantigens not present in multiplex ANA tests. 7 8 • Many commercial laboratories and some hospital laboratories have switched their ANA screening 9 test to solid phase immunoassays, such as a multiplex platform. The latter technique can screen 10 and process large volumes of clinical specimens more quickly and at less cost than the traditional 11 immunofluorescence ANA test using fixed HEp-2 cells as substrate. 12 13 • These multiplex assays can detect only the specific autoantibodies directed against the limited 14 number (typically 8-10) autoantigens that are displayed. 15 16 • Laboratories should indicate the method used when reporting ANA results. 17 18 BACKGROUND: 19 20 The methodology of the tests for the detection of antinuclear antibodies has changed over the years from 21 the LE cell prep, to immunofluorescence utilizing sections of various rodent organs (e.g. rat or mouse liver 22 or kidney, etc.) to cell lines, in particular HEp-2. HEp-2 cells contain approximately 100 to 150 23 autoantigens. These cells are used to detect ANA by the immunofluorescence method, in which both 24 pattern and titer can be described, and to display a variety of autoantigens not present in the multiplex ANA 25 tests. Researchers have seen the evolution of methodology of tests for the detection of particular ANAs 26 (anti-DNA, Sm, RNP, Ro/SS-A, La/SS-B, etc.) from immunodiffusion, complement-fixation, 27 hemagglutination, to various solid phase immunoassays. 28 29 Over the years, numerous investigators and commercial organizations have attempted to develop solid 30 phase immunoassays for the detection of ANA and specific ANAs, which are easier and cheaper to perform 31 and standardize compared to immunofluorescence assays using fixed HEp-2 cells as a substrate. A review 32 of the literature by the committee indicates that up to 35% of patients with SLE and a positive ANA by 33 immunofluorescence (IF) were negative on solid phase assays (1-4, 6-21, 23). Many commercial laboratories 34 and some hospital laboratories have switched their antinuclear antibody (ANA) screening test to solid 35 phase immunoassays, such as a multiplex platform, for the reasons noted above, and since the latter 36 technique can screen and process large volumes of clinical specimens than the traditional 37 immunofluorescence ANA test using fixed HEp-2 cells as substrate. 38 39 Various national and international organizations have also been involved in the standardization of these 40 tests for the harmonization of laboratory results. These include World Health Organization, Centers for 41 Disease Control, Dutch Red Cross and the International Union of Immunological Societies (5).
  • 2. 42 43 Any laboratory test, to be most useful, must maximally distinguish patients with a particular disorder from 44 related disorders. It is understood that both commercial and hospital laboratories are interested and 45 committed to providing the best laboratory tests for the diagnosis of rheumatic diseases. 46 47 The immunofluorescence ANA test is the gold standard for ANA testing. When performed with a history 48 and physical, it identifies almost all patients with systemic lupus erythematosus (sensitivity over 95%)(22), 49 although the specificity of this assay is only 57% for SLE when compared to patients with related 50 rheumatic and autoimmune disorders(22). In addition, the IF ANA is an important test for the screening and 51 diagnosis of systemic sclerosis (sensitivity 85%), polymyositis/dermatomyositis (sensitivity 61%), primary 52 Sjogren’s syndrome (sensitivity 48%), juvenile idiopathic arthritis (sensitivity 57%), drug-induced lupus 53 (sensitivity 100%), mixed connective tissue disease (sensitivity 100%), and autoimmune hepatitis as well as 54 being important in monitoring and assessing prognosis in individuals with Raynaud’s phenomenon. 55 56 57 RECOMMENDATIONS: 58 59 • The immunofluorescence (IF) ANA test should remain the gold standard for ANA testing. 60 61 • Hospital and commercial laboratories using bead-based multiplex platforms or other solid phase 62 assays for detecting ANAs must provide data to ordering physicians on request that their assay has 63 the same or improved sensitivity and specificity compared to the IF ANA. 64 65 • In-house assays for detecting ANA as well as anti-DNA, anti-Sm, anti-RNP, anti-Ro/SS-A, anti- 66 La/SS-B, etc. should be standardized according to national (e.g., CDC) and/or international (e.g., 67 WHO, IUIS) standards. 68 69 • Laboratories should specify the methods utilized for detecting ANAs when reporting their results. 70 71 REFERENCES: 72 73 1. Avaniss-Aghajani, E., Berzon, S., and Sarkissian, A. 2007. Clinical value of multiplexed bead- 74 based immunoassays for detection of autoantibodies to nuclear antigens. Clin Vaccine Immunol 75 14:505-509. 76 2. Bernardini, S., Infantino, M., Bellincampi, L., Nuccetelli, M., Afeltra, A., Lori, R., Biroccio, A., 77 Urbani, A., and Federici, G. 2004. Screening of antinuclear antibodies: comparison between 78 enzyme immunoassay based on nuclear homogenates, purified or recombinant antigens and 79 immunofluorescence assay. Clin Chem Lab Med 42:1155-1160. 80 3. Biagini, R.E., Parks, C.G., Smith, J.P., Sammons, D.L., and Robertson, S.A. 2007. Analytical 81 performance of the AtheNA MultiLyte ANA II assay in sera from lupus patients with multiple 82 positive ANAs. Anal Bioanal Chem 388:613-618. 83 4. Bonilla, E., Francis, L., Allam, F., Ogrinc, M., Neupane, H., Phillips, P.E., and Perl, A. 2007. 84 Immunofluorescence microscopy is superior to fluorescent beads for detection of antinuclear 85 antibody reactivity in systemic lupus erythematosus patients. Clin Immunol 124:18-21. 86 5. Bossuyt et al Ann Rheum Dis 2008; 67:1061-1063 87 6. Caramaschi, P., Ruzzenente, O., Pieropan, S., Volpe, A., Carletto, A., Bambara, L.M., and Biasi, 88 D. 2007. Determination of ANA specificity using multiplexed fluorescent microsphere 89 immunoassay in patients with ANA positivity at high titres after infliximab treatment: preliminary 90 results. Rheumatol Int 27:649-654. 91 7. Case Records of the Mass General Hospital. Case 5-2009: A 47-year-old woman with a rash and 92 numbness and pain in the legs. New Engl J Med 2009; 360:7---720. 93 8. Copple, S.S., Martins, T.B., Masterson, C., Joly, E., and Hill, H.R. 2007. Comparison of three 94 multiplex immunoassays for detection of antibodies to extractable nuclear antibodies using 95 clinically defined sera. Ann N Y Acad Sci 1109:464-472.
  • 3. 96 9. Eissfeller, P., Sticherling, M., Scholz, D., Hennig, K., Luttich, T., Motz, M., and Kromminga, A. 97 2005. Comparison of different test systems for simultaneous autoantibody detection in connective 98 tissue diseases. Ann N Y Acad Sci 1050:327-339. 99 10. Ghillani, P., Rouquette, A.M., Desgruelles, C., Hauguel, N., Le Pendeven, C., Piette, J.C., and 100 Musset, L. 2007. Evaluation of the LIAISON ANA screen assay for antinuclear antibody testing in 101 autoimmune diseases. Ann N Y Acad Sci 1109:407-413. 102 11. Gniewek RA, Stites DP, McHugh TM, Hilton JF, Nakagawa M. Comparison of antinuclear 103 antibody testing methods: immunofluorescence assay versus enzyme immunoassay. Clin Diagn 104 Lab Immunol. 1997 Mar;4(2):185-8. 105 12. Gonzalez, C., Garcia-Berrocal, B., Perez, M., Navajo, J.A., Herraez, O., and Gonzalez-Buitrago, 106 J.M. 2005. Laboratory screening of connective tissue diseases by a new automated ENA screening 107 assay (EliA Symphony) in clinically defined patients. Clin Chim Acta 359:109-114. 108 13. Homburger HA, Cahen YD, Griffiths J, Jacob GL. Detection of antinuclear antibodies: 109 comparative evaluation of enzyme immunoassay and indirect immunofluorescence methods.Arch 110 Pathol Lab Med. 1998 Nov;122(11):993-9. 111 14. Lopez-Hoyos, M., Rodriguez-Valverde, V., and Martinez-Taboada, V. 2007. Performance of 112 antinuclear antibody connective tissue disease screen. Ann N Y Acad Sci 1109:322-329. 113 15. Martins, T.B., Burlingame, R., von Muhlen, C.A., Jaskowski, T.D., Litwin, C.M., and Hill, H.R. 114 2004. Evaluation of multiplexed fluorescent microsphere immunoassay for detection of 115 autoantibodies to nuclear antigens. Clin Diagn Lab Immunol 11:1054-1059. 116 16. Nifli, A.P., Notas, G., Mamoulaki, M., Niniraki, M., Ampartzaki, V., Theodoropoulos, P.A., 117 Kopnitsky, M.J., and Castanas, E. 2006. Comparison of a multiplex, bead-based fluorescent assay 118 and immunofluorescence methods for the detection of ANA and ANCA autoantibodies in human 119 serum. J Immunol Methods 311:189-197. 120 17. Nossent, H., and Rekvig, O.P. 2001. Antinuclear antibody screening in this new millennium: 121 farewell to the microscope? Scand J Rheumatol 30:123-126; discussion 127-128. 122 18. Olaussen, E., and Rekvig, O.P. 1999. Screening tests for antinuclear antibodies (ANA): selective 123 use of central nuclear antigens as a rational basis for screening by ELISA. J Autoimmun 13:95- 124 102. 125 19. Shovman, O., Gilburd, B., Zandman-Goddard, G., Yehiely, A., Langevitz, P., and Shoenfeld, Y. 126 2005. Multiplexed AtheNA multi-lyte immunoassay for ANA screening in autoimmune diseases. 127 Autoimmunity 38:105-109. 128 20. Sinclair, D., Saas, M., Williams, D., Hart, M., and Goswami, R. 2007. Can an ELISA replace 129 immunofluorescence for the detection of anti-nuclear antibodies?--The routine use of anti-nuclear 130 antibody screening ELISAs. Clin Lab 53:183-191. 131 21. Smith, J., Onley, D., Garey, C., Crowther, S., Cahir, N., Johanson, A., Painter, S., Harradence, G., 132 Davis, R., and Swarbrick, P. 2005. Determination of ANA specificity using the UltraPlex 133 platform. Ann N Y Acad Sci 1050:286-294. 134 22. Solomon et al. Evidence-based guidelines for the use of immunologic testing: ANA. Arth Care 135 Res 2002;47:434-444. 136 23. Ulvestad, E. 2001. Performance characteristics and clinical utility of a hybrid ELISA for detection 137 of ANA. Apmis 109:217-222. 138 139 140 Approved by the Committee on Rheumatologic Care: 01/2009 141 Approved by the Board of Directors: 02/2009