Range of antinuclear antibodies in 'healthy' individuals

E. M. Tan; T. E.W. Feltkamp; J. S. Smolen; B. Butcher; R. Dawkins; M. J. Fritzler; T. Gordon; J. A. Hardin; J. R. Kalden; R. G. Lahita; R. N. Maini; J. S. McDougal; N. F. Rothfield; R. J. Smeenk; Y. Takasaki; A. Wiik; M. R. Wilson; J. A. Koziol

doi:10.1002/art.1780400909

Range of antinuclear antibodies in 'healthy' individuals

E. M. Tan, T. E.W. Feltkamp, J. S. Smolen, B. Butcher, R. Dawkins, M. J. Fritzler, T. Gordon, J. A. Hardin, J. R. Kalden, R. G. Lahita, R. N. Maini, J. S. McDougal, N. F. Rothfield, R. J. Smeenk, Y. Takasaki, A. Wiik, M. R. Wilson, J. A. Koziol

Research output: Contribution to journal › Article › peer-review

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Abstract

Objective. To determine the range of antinuclear antibodies (ANA) in 'healthy' individuals compared with that in patients with systemic lupus erythematosus (SLE), systemic sclerosis (SSc; scleroderma), Sjogren's syndrome (SS), rheumatoid arthritis (RA), or soft tissue rheumatism (STR). Methods. Fifteen international laboratories experienced in performing tests for ANA by indirect immunofluorescence participated in analyzing coded sera from healthy individuals and from patients in the 5 different disease groups described above. Except for the stipulation that HEp-2 cells should be used as substrate, each laboratory used its own in-house methodology so that the data might be expected to reflect the output of a cross-section of worldwide ANA reference laboratories. The sera were analyzed at 4 dilutions: 1:40, 1:80, 1:160, and 1:320. Results. In healthy individuals, the frequency of ANA did not differ significantly across the 4 age sub-groups spanning 20-60 years of age. This putatively normal population was ANA positive in 31.7% of individuals at 1:40 serum dilution, 13.3% at 1:80, 5.0% at 1:160, and 3.3% at 1:320. In comparison with the findings among the disease groups, a low cutoff point at 1:40 serum dilution (high sensitivity, low specificity) could have diagnostic value, since it would classify virtually all patients with SLE, SSc, or SS as ANA positive. Conversely, a high positive cutoff at 1:160 serum dilution (high specificity, low sensitivity) would be useful to confirm the presence of disease in only a portion of cases, but would be likely to exclude 95% of normal individuals. Conclusion. It is recommended that laboratories performing immunofluorescent ANA tests should report results at both the 1:40 and 1:160 dilutions, and should supply information on the percentage of normal individuals who are positive at these dilutions. A low- titer ANA is not necessarily insignificant and might depend on at least 4 specific factors. ANA assays can be a useful discriminant in recognizing certain disease conditions, but can create misunderstanding when the limitations are not fully appreciated.

Original language	English (US)
Pages (from-to)	1601-1611
Number of pages	11
Journal	Arthritis and Rheumatism
Volume	40
Issue number	9
DOIs	https://doi.org/10.1002/art.1780400909
State	Published - Sep 1997
Externally published	Yes

ASJC Scopus subject areas

Immunology and Allergy
Rheumatology
Immunology
Pharmacology (medical)

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10.1002/art.1780400909

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Tan, E. M., Feltkamp, T. E. W., Smolen, J. S., Butcher, B., Dawkins, R., Fritzler, M. J., Gordon, T., Hardin, J. A., Kalden, J. R., Lahita, R. G., Maini, R. N., McDougal, J. S., Rothfield, N. F., Smeenk, R. J., Takasaki, Y., Wiik, A., Wilson, M. R., & Koziol, J. A. (1997). Range of antinuclear antibodies in 'healthy' individuals. Arthritis and Rheumatism, 40(9), 1601-1611. https://doi.org/10.1002/art.1780400909

Tan, EM, Feltkamp, TEW, Smolen, JS, Butcher, B, Dawkins, R, Fritzler, MJ, Gordon, T, Hardin, JA, Kalden, JR, Lahita, RG, Maini, RN, McDougal, JS, Rothfield, NF, Smeenk, RJ, Takasaki, Y, Wiik, A, Wilson, MR & Koziol, JA 1997, 'Range of antinuclear antibodies in 'healthy' individuals', Arthritis and Rheumatism, vol. 40, no. 9, pp. 1601-1611. https://doi.org/10.1002/art.1780400909

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title = "Range of antinuclear antibodies in 'healthy' individuals",

abstract = "Objective. To determine the range of antinuclear antibodies (ANA) in 'healthy' individuals compared with that in patients with systemic lupus erythematosus (SLE), systemic sclerosis (SSc; scleroderma), Sjogren's syndrome (SS), rheumatoid arthritis (RA), or soft tissue rheumatism (STR). Methods. Fifteen international laboratories experienced in performing tests for ANA by indirect immunofluorescence participated in analyzing coded sera from healthy individuals and from patients in the 5 different disease groups described above. Except for the stipulation that HEp-2 cells should be used as substrate, each laboratory used its own in-house methodology so that the data might be expected to reflect the output of a cross-section of worldwide ANA reference laboratories. The sera were analyzed at 4 dilutions: 1:40, 1:80, 1:160, and 1:320. Results. In healthy individuals, the frequency of ANA did not differ significantly across the 4 age sub-groups spanning 20-60 years of age. This putatively normal population was ANA positive in 31.7% of individuals at 1:40 serum dilution, 13.3% at 1:80, 5.0% at 1:160, and 3.3% at 1:320. In comparison with the findings among the disease groups, a low cutoff point at 1:40 serum dilution (high sensitivity, low specificity) could have diagnostic value, since it would classify virtually all patients with SLE, SSc, or SS as ANA positive. Conversely, a high positive cutoff at 1:160 serum dilution (high specificity, low sensitivity) would be useful to confirm the presence of disease in only a portion of cases, but would be likely to exclude 95% of normal individuals. Conclusion. It is recommended that laboratories performing immunofluorescent ANA tests should report results at both the 1:40 and 1:160 dilutions, and should supply information on the percentage of normal individuals who are positive at these dilutions. A low- titer ANA is not necessarily insignificant and might depend on at least 4 specific factors. ANA assays can be a useful discriminant in recognizing certain disease conditions, but can create misunderstanding when the limitations are not fully appreciated.",

author = "Tan, {E. M.} and Feltkamp, {T. E.W.} and Smolen, {J. S.} and B. Butcher and R. Dawkins and Fritzler, {M. J.} and T. Gordon and Hardin, {J. A.} and Kalden, {J. R.} and Lahita, {R. G.} and Maini, {R. N.} and McDougal, {J. S.} and Rothfield, {N. F.} and Smeenk, {R. J.} and Y. Takasaki and A. Wiik and Wilson, {M. R.} and Koziol, {J. A.}",

year = "1997",

month = sep,

doi = "10.1002/art.1780400909",

language = "English (US)",

volume = "40",

pages = "1601--1611",

journal = "Arthritis and Rheumatism",

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TY - JOUR

T1 - Range of antinuclear antibodies in 'healthy' individuals

AU - Tan, E. M.

AU - Feltkamp, T. E.W.

AU - Smolen, J. S.

AU - Butcher, B.

AU - Dawkins, R.

AU - Fritzler, M. J.

AU - Gordon, T.

AU - Hardin, J. A.

AU - Kalden, J. R.

AU - Lahita, R. G.

AU - Maini, R. N.

AU - McDougal, J. S.

AU - Rothfield, N. F.

AU - Smeenk, R. J.

AU - Takasaki, Y.

AU - Wiik, A.

AU - Wilson, M. R.

AU - Koziol, J. A.

PY - 1997/9

Y1 - 1997/9

N2 - Objective. To determine the range of antinuclear antibodies (ANA) in 'healthy' individuals compared with that in patients with systemic lupus erythematosus (SLE), systemic sclerosis (SSc; scleroderma), Sjogren's syndrome (SS), rheumatoid arthritis (RA), or soft tissue rheumatism (STR). Methods. Fifteen international laboratories experienced in performing tests for ANA by indirect immunofluorescence participated in analyzing coded sera from healthy individuals and from patients in the 5 different disease groups described above. Except for the stipulation that HEp-2 cells should be used as substrate, each laboratory used its own in-house methodology so that the data might be expected to reflect the output of a cross-section of worldwide ANA reference laboratories. The sera were analyzed at 4 dilutions: 1:40, 1:80, 1:160, and 1:320. Results. In healthy individuals, the frequency of ANA did not differ significantly across the 4 age sub-groups spanning 20-60 years of age. This putatively normal population was ANA positive in 31.7% of individuals at 1:40 serum dilution, 13.3% at 1:80, 5.0% at 1:160, and 3.3% at 1:320. In comparison with the findings among the disease groups, a low cutoff point at 1:40 serum dilution (high sensitivity, low specificity) could have diagnostic value, since it would classify virtually all patients with SLE, SSc, or SS as ANA positive. Conversely, a high positive cutoff at 1:160 serum dilution (high specificity, low sensitivity) would be useful to confirm the presence of disease in only a portion of cases, but would be likely to exclude 95% of normal individuals. Conclusion. It is recommended that laboratories performing immunofluorescent ANA tests should report results at both the 1:40 and 1:160 dilutions, and should supply information on the percentage of normal individuals who are positive at these dilutions. A low- titer ANA is not necessarily insignificant and might depend on at least 4 specific factors. ANA assays can be a useful discriminant in recognizing certain disease conditions, but can create misunderstanding when the limitations are not fully appreciated.

AB - Objective. To determine the range of antinuclear antibodies (ANA) in 'healthy' individuals compared with that in patients with systemic lupus erythematosus (SLE), systemic sclerosis (SSc; scleroderma), Sjogren's syndrome (SS), rheumatoid arthritis (RA), or soft tissue rheumatism (STR). Methods. Fifteen international laboratories experienced in performing tests for ANA by indirect immunofluorescence participated in analyzing coded sera from healthy individuals and from patients in the 5 different disease groups described above. Except for the stipulation that HEp-2 cells should be used as substrate, each laboratory used its own in-house methodology so that the data might be expected to reflect the output of a cross-section of worldwide ANA reference laboratories. The sera were analyzed at 4 dilutions: 1:40, 1:80, 1:160, and 1:320. Results. In healthy individuals, the frequency of ANA did not differ significantly across the 4 age sub-groups spanning 20-60 years of age. This putatively normal population was ANA positive in 31.7% of individuals at 1:40 serum dilution, 13.3% at 1:80, 5.0% at 1:160, and 3.3% at 1:320. In comparison with the findings among the disease groups, a low cutoff point at 1:40 serum dilution (high sensitivity, low specificity) could have diagnostic value, since it would classify virtually all patients with SLE, SSc, or SS as ANA positive. Conversely, a high positive cutoff at 1:160 serum dilution (high specificity, low sensitivity) would be useful to confirm the presence of disease in only a portion of cases, but would be likely to exclude 95% of normal individuals. Conclusion. It is recommended that laboratories performing immunofluorescent ANA tests should report results at both the 1:40 and 1:160 dilutions, and should supply information on the percentage of normal individuals who are positive at these dilutions. A low- titer ANA is not necessarily insignificant and might depend on at least 4 specific factors. ANA assays can be a useful discriminant in recognizing certain disease conditions, but can create misunderstanding when the limitations are not fully appreciated.

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Range of antinuclear antibodies in 'healthy' individuals

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