Hormone Immunoassay Interference: A 2021 Update.

Immunoassays are powerful qualitative and quantitative analytical techniques. Since the first description of an immunoassay method in 1959, advances have been made in assay designs and analytical characteristics, opening the door for their widespread implementation in clinical laboratories. Clinical endocrinology is closely linked to laboratory medicine because hormone quantification is important for the diagnosis, treatment, and prognosis of endocrine disorders. Several interferences in immunoassays have been identified through the years; although some are no longer encountered in daily practice, cross-reaction, heterophile antibodies, biotin, and anti-analyte antibodies still cause problems. Newer interferences are also emerging with the development of new therapies. The interfering substance may be exogenous (e.g., a drug or substance absorbed by the patient) or endogenous (e.g., antibodies produced by the patient), and the bias caused by interference can be positive or negative. The consequences of interference can be deleterious when clinicians consider erroneous results to establish a diagnosis, leading to unnecessary explorations or inappropriate treatments. Clinical laboratories and manufacturers continue to investigate methods for the detection, elimination, and prevention of interferences. However, no system is completely devoid of such incidents. In this review, we focus on the analytical interferences encountered in daily practice and possible solutions for their detection or elimination.

INTRODUCTION

Immunoassays are widely used in clinical laboratories for a variety of hormone analyses. Since the first insulin immunoassay described by Berson and Yalow (which received the 1977 Nobel Prize in Medicine), immunoassays have evolved considerably [1]. However, with widespread adaptation of these techniques, several interferences have been identified. Immunoassays are susceptible to interference because of the complexities of the antigen (Ag)–antibody (Ab) interaction occurring in a complex matrix [2]. Such interference leads to incorrect interpretation of immunoassay results, leading to unnecessary explorations or administration of inappropriate therapy.

Immunoassay design initially relied on the development of polyclonal Abs obtained from animal sources in a competitive format; In 1975, Köhler and Milstein [3] described the monoclonal Ab (mAb) development technique (which received the 1984 Nobel Prize in Medicine), leading to the development of non-competitive (sandwich) immunoassays where two different mAbs can recognize the same Ag in one incubation step. The sensitivity and specificity of immunoassays made it possible to detect and quantify analytes at extremely low concentrations, which was not possible with other clinical chemistry techniques. Along with the advantages of a rapid measurement time and fully automated instruments, the improved analytical performance led to immunoassays becoming a widely adopted technique in clinical laboratories.

Analytical systems have been developed to be more rapid and efficient with advantages of the automation evolution to meet the demands of an augmented workload and the need for rapid analysis. However, these advancements are associated with drawbacks such as the low specificity of direct steroid immunoassays.The systems have also become more reliable owing to improvements in immunoassay reagents and signal detection systems.

These advances have decreased, but not completely eliminated, the incidence of interference in immunoassays. Analytical errors from endogenous interferents still occur with some patient samples [4]. Interference might induce false-positive results, false-negative results, or both, which can simulate a seemingly coherent hormonal profile that might drive unnecessary explorations, inappropriate treatments, or a missed diagnosis.

Laboratory quality control efforts (i.e., compliance with regulatory and accreditation demands, instrument maintenance, internal and external evaluation programs) have an ultimate goal of rapidly obtaining reliable and accurate results. However, interferents in patient samples are not detectable by standard quality control procedures and are reproducible within a given analytical system [5]. Laboratory specialists must take a critical view of results and not blindly trust the instruments. Knowledge of physiology and normal variations in biological markers enables assessing whether discordance with previous results is acceptable, or for identification of an aberrant result in some cases. Precise understanding of the analytical principles and assay design is also necessary for the correct interpretation of laboratory results and suspicion of erroneous results.

In this review, we discuss the types of immunoassays commonly used in laboratories, the mechanisms involved in possible in vitro analytical interference, and the solutions and strategies employed to suspect and overcome such interference, including recently reported emerging interferences. Hormone concentrations modification by the pharmacological action of a drug is beyond the scope of this review and will not be addressed.

METHODS USED IN HORMONE ASSAYS

There are two main methodologies widely used in hormonology laboratories: immunoassay methods and mass spectrometry methods. In this review, we exclusively focus on immunoassays, which can be classified into competitive and non-competitive (sandwich) immunoassays.

Competitive (limited reagent) immunoassays

In competitive immunoassays, the analyte (Ag) competes with a signal-labeled Ag (tracer) for limited quantities of Ab (Fig. 1A). After a washing step, the bound signal is produced and the analyte concentration in the sample is inversely correlated with the generated signal. These assays can be performed either simultaneously (the majority), where both the patient sample and labeled Ag are added at the same time, or sequentially, where the labeled Ag is added in a second step after allowing the Ab–Ag reaction to reach equilibrium.

Fig. 1

Two types of immunoassays. (A) Competitive immunoassay. The sample is incubated with an anti-cortisol antibody (Ab) (for example), and a tracer (cortisol labeled with a measurable signal: enzyme, fluorescent, or luminescent compound isotope) is added. Competition occurs between the cortisol in the sample and the labeled cortisol for the Ab-binding sites. These cortisol molecules bound to the Ab are captured on a solid phase. Unlike sandwich assays, the higher the cortisol concentration in the sample, the lower the signal-labeled cortisol bound to the antibody and finally linked to the solid phase. (B) Sandwich immunoassay. TSH (for example) is “sandwiched” between two different antibodies: one is labeled with a signal to be measured (luminescent or fluorescent compound, enzyme, isotope) and the other one, named the “capture antibody,” will allow the separation of the immune complexes on a solid phase. The higher the TSH concentration, the higher the signal linked to the solid phase will be.

Abbreviations: Ab, antibody; Ag, antigen; TSH, thyroid-stimulating hormone.

Non-competitive/sandwich or “two-sites” (excess reagent) immunoassays

In non-competitive immunoassays, the capture Ab is fixed on a solid phase, and then the analyte (in the sample) and labeled Ab (tracer) are added (Fig. 1B). The two Abs recognize different epitopes on the analyte. The capture and labeled Abs can be monoclonal, polyclonal, or both. After a washing step, the tracer signal is produced and the analyte concentration in the sample is directly correlated with the generated signal.

Competitive versus sandwich assays

The majority of hormone immunoassays are heterogeneous; thus, the choice of methodology for immune complex separation is specific to each reagent manufacturer and each analyte. In competitive and sandwich immunoassays, the capture Ab must be separated from the reaction mixture at the end of the reaction. This is facilitated either by a solid-phase coating of the capture Ab or by using a biotinylated Ab (or biotinylated Ag), which will be captured by a streptavidin solid phase. Other methods use a solid phase-coated Ab directed against the capture Ab specific to the analyte (separation step using a second Ab).

Sandwich immunoassays are suitable for larger molecules [e.g., polypeptide hormones, pituitary hormones, parathyroid hormone (PTH), calcitonin, thyroglobulin (Tg), insulin, C-peptide, insulin-like growth factor 1 (IGF-1), proteins, anti-Müllerian hormone (AMH), inhibin], whereas competitive immunoassays are better suited for detecting smaller molecules because only one antigenic site will be recognized by one Ab [e.g., thyroid hormones T3 and T4 (either total or free), steroids, 25 hydroxy vitamin D] [6]. Many assays for Ab detection and quantification are also designed according to the “competitive” format [Ab to thyroid-stimulating hormone (TSH) receptor, anti-thyroid peroxidase, and anti-Tg].

Both competitive and sandwich immunoassays have their advantages and pitfalls. Competitive immunoassays are mandatory for small molecules but are susceptible to cross-reactions with precursors or metabolites of the analyte or with drugs, and to interference from endogenous Abs and biotin when the biotin–streptavidin complex is used to separate the immunocomplex. Sandwich immunoassays are usually more robust since Ab reagents are introduced in excess. Sandwich immunoassays also present higher specificity and a lower limit of quantification; however, these assays are prone to some interference due to endogenous Abs, biotin, and the hook effect, which is specific to the sandwich format.

TYPES OF INTERFERENCE

Pre-analytical factors

Obtaining reliable laboratory results begins at the sample collection stage. Pre-analytical conditions have to be respected, such as the tube type (serum vs. plasma, type of anti-coagulant for plasma, with or without a separating gel); time of collection for hormones with time-dependent concentrations (e.g., cortisol and testosterone concentrations are higher in the morning and estradiol concentrations depend on the day in the menstrual cycle); storage and transportation temperature [adrenocorticotropic hormone (ACTH) at +4°C, renin at 20–25°C]; and the absence of hemolysis (insulin) [7-9]. Bilirubin and lipids can also interfere with immunoassays, depending on the immunoassay design and signal detection system.

Azides are commonly used as preservatives for long-term storage, but they have been shown to destroy peroxidase labels. EDTA is a powerful chelating agent that binds to the metallic ions of labels (e.g., europium) or to the cofactor required for some enzymes’ activity (e.g., zinc for alkaline phosphatase) [10]. Since samples stored in EDTA require more caution than serum regarding the risk of signal interference, serum is the matrix of choice for many analytes.

Cross-reaction/assay specificity

The presence of molecules structurally related to the Ag within the biological sample might lead to a cross-reaction and unwanted recognition by the Ab, leading to specificity problems. These cross-reactants can be either metabolites or precursors of the analyte or drugs (either native or drug metabolites). Some classical examples of such challenging interference are presented in Table 1, together with recent drugs leading to specificity problems such as fulvestrant (in estradiol immunoassays) and pegvisomant, a growth hormone (GH) analog and receptor antagonist (in GH immunoassays).

Table 1

Common problems of cross-reaction and specificity in current immunoassays

Analyte	Cross-reacting compound	Context	Reference
Competitive immunoassays
17OH progesterone	17OH pregnenolone sulfate	Neonates (especially preterm)	Wong, et al. 1992 [182]Makela and Ellis, 1988 [183]
Cortisol	11 desoxy cortisol	11 Hydroxylase defectMetyrapone test	Ward, et al. 2017 [26]Hawley, et al. 2016 [184]
	Prednisone, prednisolone and methylprednisolone	Corticoid therapy	Ward, et al. 2017 [26]Vogeser, et al. 2017 [185]
Estradiol	Estrone sulfate	Hormone replacement therapy (oral administration)	Thomas, et al. 1993 [186]
	Fulvestrant	Breast cancer therapy	Owen, et al. 2019 [11]
	Exemestane metabolites	Breast cancer therapy	Mandic, et al. 2017 [12]
Progesterone	Di-hydroprogesterone	Micronized progesterone therapy	Nahoul, et al. 1987 [187]
Testosterone	Fetal and placental steroids	Females, children	Taieb, et al. 2003 [188]Honour, 2010 [17]
Testosterone	DHEA-S	Females	Warner, et al. 2006 [189]
T3 (either total or free)	Triiodoacetic acid		Piketty, et al. 1996 [190]
DHEAS	Pregnenolone sulphate	Pregnancy	Krasowski, et al. 2014 [191]
Sandwich immunoassays
ACTH 1-39	Fragments, precursor	Paraneoplastic tumors	Raff and Findling, 1989 [20]
Insulin	Pharmacological analogs	Inappropriate injection leading to hypoglycemia	Parfitt, et al. 2015 [22]Giurgea, et al. 2005 [24]Dayaldasani, et al. 2015 [23]
Growth hormone	Pegvisomant	Acromegaly therapy	Paisley, et al. 2007 [18]Manolopoulou, et al. 2012 [19]
	Placental GH	Pregnancy	Dias, et al. 2013 [192]

Abbreviations: ACTH, adrenocorticotropic hormone; DHEAS, dehydroepiandrosterone sulfate.

Biochemical evaluation of menopausal status with accurate estradiol concentration measurements are needed for establishing the treatment strategy in patients with estrogen receptor-positive breast cancer. Fulvestrant is a selective estrogen receptor antagonist that triggers degradation of the receptor. In breast cancer patients, fulvestrant leads to marked cross-reactions in estradiol immunoassays because of structural similarities (the long half-life of fulvestrant leads to interference lasting for months in these patients) [11]. Likewise, the aromatase inhibitor exemestane is a structural analog of estradiol prescribed in breast cancer therapy. Biochemical evaluations of estradiol in exemestane therapy cause false-positive results in most estradiol immunoassays because of cross-reaction with exemestane metabolites [12].

The presence of a cross-reactant can lead to inaccurate results depending on the assay format, with competitive immunoassays being the most susceptible to this problem. In a competitive immunoassay, the cross-reactant usually induces a false increase (except in one estriol immunoassay, owing to a particular design [13]). Notably, direct steroid immunoassays (without an extraction step of the sample with an organic solvent) can be affected by cross-reaction (e.g., cortisol metabolites, synthetic glucocorticoids in cortisol immunoassays) [14]. In testosterone concentration measurements, second-generation immunoassays avoid dehydroepiandrosterone sulfate (DHEAS) cross-reaction [15, 16]. However, an extraction step prior to the immunoassay is required for samples from women and children to protect against other cross-reactants [17].

For molecules large enough to bear two unhindered specific epitopes, two-site sandwich assays exhibit superior specificity to that of competitive assays. Interference is less frequent in a sandwich immunoassay because of double epitope recognition. However, its manifestation will depend on the epitopes involved in sandwich formation; if both the capture and signal Abs bind a structurally related cross-reactant, a false increase will occur (e.g., pegvisomant for some GH assays) [18, 19]. Conversely, if only one Ab (either the capture or signal Ab) attaches to the structurally related cross-reactant, a false decrease will be obtained, because the sandwich complex will not be completed and the signal Ab will be washed away after the separation step [18]. In some cases, it is clinically important to detect precursors or fragments present in certain tumors, together with the intact form of the hormone such as ACTH [20, 21]. High specificity for intact pituitary ACTH 1-39 is not always desirable. Another example is insulin immunoassays, where recognition of insulin pharmacological analogs can be useful in the rare cases of surreptitious administration [22-24]. The lack of recognition of all hormone isoforms can also be deleterious in some cases such as TSH immunoassays that do not recognize variants present in some ethnic groups [25].

A lack of or too high specificity can, in some circumstances, lead to inaccurate results. Wide specificity can be of great value, depending on the clinical context, which will define the appropriate specificity; the choice of epitopes to be detected is crucial and will depend on the clinical utilization of the assay. Reagent manufacturers are continuously selecting new Abs to reduce specificity problems and improve their immunoassays [26]. In any case, appropriate interpretation of the result depends on the knowledge regarding assay specificity.

The hook effect

This phenomenon may occur in sandwich immunoassays when measuring very high hormone concentrations; the hook effect occurs specifically in progressive tumor pathologies, in which the magnitude of variation between the physiological and pathological concentrations can be extreme (such as in prolactinoma, thyroid carcinoma, and hydatiform moles). To our knowledge, the hook effect has never been described in cases of somatotropinomas (acromegaly) or corticotropinomas (Cushing disease), possibly because these tumors are rarely large enough to produce extreme hormone concentrations [27]. In two-site sandwich immunoassays, the excess Ag might prevent sandwich formation with the capture and signal Abs separately bound to the Ag and the signal Ab being washed away, resulting in an apparently lower concentration (Fig. 2). This could result in delayed diagnosis and treatment for serious conditions, or even misdiagnosis with serious consequences. For example, an unrecognized hook effect can result in erroneous diagnosis of a non-functioning pituitary tumor, subjecting the patient to unnecessary surgery instead of prescribing dopamine agonists (in the case of macroprolactinoma) [28]. The hook effect impacts only sandwich immunoassays, and sample dilution will reveal the presence of excess analyte; with serial dilutions, the concentration of the analyte will increase until two coherent successive dilutions are obtained. Manufacturers tend to use excess Abs or reduce the required sample volume to minimize possible Ab saturation and the frequency of the hook effect. Table 2 presents recent examples of reported cases of the hook effect for hormone concentration measurements.

Fig. 2

The hook effect in sandwich immunoassays. The excess Ag saturates both capture and labeled Abs; no or little amount of the Ab–Ag–Ab complex is formed, leading to false low results.

Abbreviations: Ab, antibody; Ag, antigen.

Table 2

Examples of reported cases of the hook effect for hormone measurements

Analyte	Measured concentration before dilution	Actual concentration after serial dilution	Reference
Prolactin	164.5 ng/mL	26,000 ng/mL (macroadenoma)	Frieze, et al. 2002 [28]
Calcitonin	182 ng/L	450,000 ng/L	Schiettecatte, et al. 2016 [193]
Thyroglobulin	3.8 ng/mL 4.6 ng/mL	207,855 ng/mL 140,462 ng/mL	Hillebrand, et al. 2020 [194]
HCG	Low/normal	5,899,478 mIU/mL (gestational trophoblastic disease)	Cormano, et al. 2015 [195]

Abbreviation: HCG, human chorionic gonadotropin.

Interfering Abs

Endogenous interfering Abs are highly heterogeneous in nature and in their interference mechanisms. The problem induced by endogenous Abs that can inhibit either the Ag–Ab complex separation (at the end of incubation in the reaction mixture) or the signal development will be addressed in subsequent sections (Their impact on these steps gives them the ability to affect multiple immunoassays simultaneously in a bidirectional way). This section discusses other interfering Abs, including those affecting immunocomplex formation or analyte recognition, directed against animal reagent Abs or the analyte itself.

Heterophile Abs and anti-animal Abs

Heterophile Abs are polyclonal Abs found in human samples that can react with assay reagent Abs obtained from different species. They may lead to false high (mostly) or false low results. Studies on the prevalence of this interference in immunoassays have yielded values ranging from 0.4% to 0.5% [29, 30].

The definition of heterophile and human anti-animal Abs [HAAA; mostly human anti-mouse Abs (HAMAs)] is confusing and overlapping among studies, because some authors have used the term “heterophilic Ab” to refer to any endogenous interfering Ab, regardless of the mechanism. Heterophile Abs are typically of human origin, endogenous, and weakly poly-specific Abs; they are considered to occur naturally and are able to react with Abs from multiple species. In contrast, HAAAs are monospecific, high-affinity Abs, which can appear after exposure to animals or animal products, viral or bacterial infections, in an autoimmune clinical context, or without any identified cause. Their interference mechanism is, however, similar to that of heterophile antibodies. In laboratory practice, the term “heterophile Ab” is typically used whenever an endogenous Ab is suspected to bind to the assay Abs [29, 31]. Knowledge of previous exposure to diagnostic or therapeutic Abs is important; the term “heterophile” should theoretically be used only when there is no evidence of exposure to animal Ig [31, 32]. Heterophile Abs can be of the IgG, IgM, or IgA isotype. Although they bind mostly to the Fc region of the assay Abs, there are reports of these interfering Abs binding to other parts of the assay Abs (such as the idiotope or the hinge region) [33, 34].

The Ab interference mechanism varies depending on the assay design. In sandwich immunoassays, a heterophile Ab can form a bridge between capture and labeled Abs (cross-linking the two Abs), resulting in false-positive interference in most cases (Fig. 3A-1) [35]. Rarely, a heterophile Ab can prevent formation of the Ag–Ab complex by binding and blocking only one of the assay Abs, preventing binding of the analyte through steric effects, resulting in false-negative interference (Fig. 3A-2) [32, 36]. Although this interference mostly concerns sandwich immunoassays, in competitive immunoassays, the interfering Ab can also give false high results by blocking the capture Ab (thus decreasing the assay signal) (Fig. 3B) or false low results [37-39]. In rare cases, heterophilic Ab interference can affect multiple hormone immunoassays simultaneously [37, 39-41].

Fig. 3

Mechanisms of Ab interference in immunoassays. (A) In sandwich immunoassays, the Ab can (1) cross-link the capture and detection Abs (false positive), and (2, 3) prevent the formation of the Ab–Ag–Ab complex by blocking the Abs or the analyte (false negative). (B) In competitive immunoassays, the Ab can block the capture Ab or the analyte giving false high results.

Abbreviations: Ab, antibody; Ag, antigen.

HAAAs differ from heterophile Abs by being theoretically specific to a species and having higher avidity. Anti-animal Abs (IgG, IgM, IgA class, anti-isotype, and anti-idiotype specificity) include human anti-mouse, anti-rabbit, anti-goat, anti-sheep, anti-cow, anti-pig, anti-rat, and anti-horse Abs, and those with mixed specificity [32]. HAAAs can be transient, lasting from a few days to several months or years [42, 43]. These arise because of iatrogenic and non-iatrogenic causes of exposure to animal Ags. The exposure can happen to a variety of workers, such as animal breeding facility workers, laboratory animal technicians, and butchers, as well as from pets and dietary sources [44, 45]. Since murine mAbs are used for medical purposes, HAMAs are the most commonly encountered interfering HAAA type.

The reported prevalence of HAAA interference of less than 1% might seem low, but the impact can be greater than expected when considering the prevalence of the disease being diagnosed based on the immunoassay results. Ismail [46] showed that at a 0.4% probability of analytical interference for subclinical hypothyroidism with a 2% prevalence (for both sexes at all ages), only 83% of the results are diagnostically correct, meaning that 17% of the cases will be falsely diagnosed.

There has been recent revolutionary progress in immunotherapies for treating cancers, autoimmune diseases, and other clinical conditions. As of December 2019, the United States Food and Drug Administration agency has approved 79 therapeutic mAbs [47]. This increases the possibility of Ab-related interference, because a therapeutic Ab can act as an Ag leading to the generation of HAMAs. Immune checkpoint inhibitors can induce real endocrine disorders such as dysthyroidism, hypophysitis, and adrenal insufficiency, and thus represent a crucial problem. The discordant clinical picture with laboratory results raises the question of possible interference in immunoassays, especially when the mAb used in treatment is not completely humanized; the probability of detecting HAAAs is theoretically 90% for a murine mAb, 40% for a chimeric mAb, and 10% for a humanized therapeutic mAb [48, 49]. In 2010, Koshida, et al. [50] developed an assay for HAMA, and recorded 11.7% positive samples among inpatients and outpatients. A very small percentage of HAMAs will produce an erroneous result. However, the number of potential errors with clinical consequences is worrisome owing to the vast number of immunoassays performed [51]. For example, Jonklaas [52] reported a case of falsely elevated free thyroxin (FT4) concentration in a patient after starting treatment with checkpoint inhibitor murine mAbs for metastatic melanoma. Interestingly, heterophile Ab interference was recently reported in PTH and Tg immunoassays for three patients after the transfer of ex vivo-expanded natural killer cells [53].

Rheumatoid factors (RFs)

RFs can interfere with immunoassays via the same mechanisms as those of heterophile Abs. RFs are predominantly of the IgM isotype, which interact with the Fc part of human IgG but can also react with that of different species with variable affinity, although their affinity seems to be low with mouse IgG [54]. RFs are found in more than 70% of patients with rheumatoid arthritis and other autoimmune diseases. The RF concentration can also increase during infection with inflammation.

RFs can be measured in suspected samples and eliminated by different techniques. Astarita, et al. [55] reported a case of interference in Tg concentration measurements in a woman with differentiated thyroid cancer and a rheumatoid arthritis history, where detectable Tg became undetectable after eliminating RFs through polyethylene glycol (PEG) treatment. RF interference can affect multiple parameters simultaneously; Mongolu, et al. [56] reported the case of a 60-year-old male patient with a history of rheumatoid arthritis, who had high serum concentrations of luteinizing hormone (LH), follicle-stimulating hormone (FSH), sex hormone-binding globulin, prolactin, human chorionic gonadotropin (HCG), and TSH. They suspected assay interference and performed further tests after eliminating RFs, which revealed normal hormone concentrations.

In most cases, comparison with alternative immunoassay results is useful when suspecting Ab interference, as the interfering Ab is most potent with the Abs of a specific class/subclass or isotype, resulting in strikingly different results with different methods [57]. Dilution tests lacking linearity, use of heterophile blocking tubes (HBTs), and protein A pretreatment are also useful to demonstrate that a result is erroneous [39]. However, no single test can be used as evidence or to rule out an erroneous result [26].

To reduce such interference, manufacturers have developed some strategies such as inclusion of non-immune animal Ig from the same species as reagent Igs, aggregated Ig, use of chimerized or humanized Abs, or two F(ab) fragments instead of intact Ig on their solid phase [26, 29]. However, heterophilic Abs are highly heterogeneous in nature, their concentrations vary largely between patients, and no blocking reagent/method is completely successful in preventing such interference. Although the frequency of heterophilic Ab interference may be declining, recent reports concerning erroneously elevated concentrations of PTH, FSH, LH, and prolactin demonstrate that this type of interference can still occur with any immunoassay [58-60].

Anti-analyte Abs and macro-analytes

Prolactin

An Ab can bind to the analyte in vivo altering its half-life and physiological role, while preserving its antigenicity, or can interfere directly with the in vitro immunoassay. Circulating monomeric prolactin can bind to IgG Abs in vivo, resulting in an inactive form with a much longer half-life, now termed “macroprolactin,” and giving higher prolactin concentrations in immunoassays. This can lead to the physician/gynecologist pursuing unnecessary explorations in approximately 4–10% of women [35, 61, 62]. The macroprolactin complex is a source of interference in prolactin immunoassays and commonly results in the misdiagnosis of hyperprolactinemia. Removal of macroprolactin by precipitation with PEG is an effective technique to identify such interference but is unfortunately not universally employed due to the manual nature of the procedure [63]. A possible explanation for the development of these anti-prolactin Abs is post-translational modifications that give rise to immunogenicity and the development of anti-prolactin autoAbs [64]. Another form of circulating prolactin is the result of auto-polymerization of prolactin in vivo, yielding large prolactin molecules that can be measured with different immunoassays. Macroprolactin can react in all prolactin immunoassays, albeit to different extents, which might be related to the degree to which the prolactin epitopes are exposed in the macroprolactin complex [35, 63, 65]. Clinical laboratories should implement a validated screening procedure to exclude macroprolactinemia in all patients presenting with hyperprolactinemia. PEG precipitation allows for the production of an Ig-free sample, which is effective in a variety of hormone immunoassays (prolactin, TSH, and FSH), resulting in at least 60% recovery. Since PEG precipitation is non-specific, some amount of the analyte is lost due to co-precipitation. PEG reduces solvent availability due to which proteins solubility is exceeded, leading to their precipitation [66]. However, the precipitation of IgA is only partial; a case of IgA macroprolactinemia with a false-negative PEG screening test was reported [63]. Since the presence of macroprolactin can change over time, an assay to detect macroprolactinemia should be repeated and macroprolactin might still develop even if it has been excluded previously [67].

Other macrohormones: macro-FSH, macro-LH, and macro-TSH

Similar to macroprolactin, macro-FSH, macro-LH, and macro-TSH can be identified, although they are less common. Macro-TSH was detected in 0.17% of infertile women with the PEG screening test, although the pathogenesis was not fully clear [68, 69]. Commercial TSH immunoassays recognize macro-TSH, resulting in a false diagnosis of hyperthyrotropinemia [35, 69]. PEG precipitation, dilution, and recovery tests could be useful in detecting this situation [70]. This finding has also been observed in euthyroid neonates due to transplacentally transmitted maternal anti-TSH Abs [71, 72].

Thyroglobulin (Tg)

In Tg immunoassays, the binding of Tg to an anti-Tg autoAb prevents the formation of many sandwich immune complexes with the assay Abs, which can underestimate Tg concentrations (Fig. 3A-3); anti-Tg Ab interference is the most serious problem currently limiting the clinical utility of Tg immunoassays [73]. Current guidelines mandate that every Tg immunoassay include anti-Tg testing, and the indirect Tg recovery approach can also be useful to detect interference, regardless of the cause [73-75].

Insulin

Insulin auto-immune hypoglycemia is an under-recognized pathology, which is common in Japanese patients (Hirata’s disease) but rarer in Caucasians [76]. Anti-insulin autoAbs have heterogeneous clinical and analytical consequences [77]. These Abs are a cause of misleading and discordant results between different insulin immunoassays (with either highly elevated or normal results). Assaying for insulin Abs is therefore needed for the differential diagnosis of hypoglycemia in non-diabetic patients [78].

Fibroblast growth factor 23 (FGF23)

The most frequent heritable disease involving FGF23 is a variant in the phosphate-regulating endopeptidase homolog X-linked (PHEX) gene, causing X-linked hypophosphatemia (XLH), with a clinical presentation of rickets/osteomalacia, growth retardation in children, demineralization, and bone pain. This loss-of-function variation leads to the upregulation of FGF23 production from the bone and resultant kidney phosphate wasting. Recently, the anti-FGF23 Ab burosumab emerged as a breakthrough therapy for XLH, targeting the chronic upregulation of FGF23. Burosumab is a fully human IgG1 mAb that binds intact FGF23. In vitro, burosumab inhibits recognition of the intact FGF23 molecule by preventing binding of one or both reagent Abs in sandwich two-site assays, indicating that the intact FGF23 molecules were no longer recognized in vitro [79].

Free thyroid hormones

The interfering anti-analyte Ab can also bind to the labeled analyte in vitro in competitive immunoassays. In one-step free thyroid hormone immunoassays, the presence of thyroid hormone autoAbs may induce spuriously elevated results (Fig. 3B-2). Immunoassays show diverse sensitivities to this pitfall, inducing variable magnitudes of interference [70, 80-82]. In vivo, the free thyroid hormone Ab seems to behave like another endogenous binding protein. The frequency of anti-T4 and anti-T3 autoAbs specifically relates to autoimmune thyroid disorders such as Hashimoto thyroiditis and other autoimmune diseases (e.g., lupus erythematosus, vitiligo) [80, 83-86]. These autoAbs can be induced by interferon-α therapy or can be transient and associated with Epstein-Barr-virus infection [87, 88]. Radiolabeled T4 (or T3) incubation followed by PEG precipitation can be useful when suspecting this type of interference [81, 82, 84].

Interference affecting immune complex separation

To help separate the reagent Abs from the reaction mixture, the streptavidin–biotin interaction is a rapid, efficient, and convenient method. The biotinylated Ab or Ag is separated on a streptavidin-linked solid phase, and this method has been widely adopted by many manufacturers. Any interferent that prevents the separation of immune complexes, will affect this interaction and potentially disturb multiple immunoassays. Either biotin or anti-streptavidin Abs (ASA) can be involved in the mechanism of this type of interference.

The biotin problem

Biotin interference has been recognized for decades, but only in the context of rare hereditary metabolic disorders [89]. However, in the last four years, the combination of the widespread use of streptavidin-biotin technology, and the more frequent therapeutic or non-therapeutic use of supraphysiological doses of biotin have led to numerous reports of erroneous hormone- and non-hormone immunoassay results [90-93]. Biotin can inhibit immune complex separation, leading to opposite erroneous results of falsely elevated or depressed hormone concentrations in competitive or sandwich immunoassays, respectively, using techniques involving streptavidin-biotin separation [90, 92, 94]. This bidirectional behavior with opposite effects may mimic an endogenous endocrine pathological condition, representing a special challenge for endocrinology assays: results seemingly consistent with a biochemical diagnosis of hyperthyroidism can be obtained indicating a “perfect storm” [falsely elevated concentrations of FT4, free T3 (FT3), anti-TSH receptor Ab, and falsely lowered TSH concentration] [91, 92]. Vitamin D intoxication, testosterone-producing tumors, hyperandrogenism, hypercorticism, or PTH suppression have also been reported as “fake news” related to high biotin intake [95-100]. Conversely, some real endocrine disorders, including primary hypothyroidism, may be missed because of biotin distortion of the assays lowering the elevated TSH concentration [89, 101, 102].

Biotin therapy can be prescribed in dermatology for the treatment of various hair, nail, and skin disorders [103]. However, there is limited clinical evidence on its efficiency, except in biotin deficiency, which is a very rare situation since biotin recommended intake of 30 μg/day is easily obtained from a normal, balanced diet [104]. Over-the-counter biotin supplements with moderately high doses (1–30 mg/day) are widely available and are now glamorized by popular media. Despite limited benefits for the treatment of hair loss or skin and nail health, the popularity of biotin appears to be important [105]. Most patients fail to mention taking this supplement to their physician, because it is not seen as a “real treatment,” and some patients are not aware of the composition of the dietary supplement. Since February 2019, the European Medicines Agency imposed including a warning message concerning the risk of erroneous laboratory results, which must accompany any biotin supplements containing biotin dose higher than 150 μg (popular vitamin cocktails, containing the usual 30 μg recommended daily intake, will not induce any in vitro laboratory distortion with any assay) [106]. The worldwide prevalence of high-biotin supplement use is not well-known but seems to be country-dependent. Some studies have evaluated the biotin concentration in patient samples from different countries. A study quantifying biotin in plasma samples from emergency department patients in the USA showed that 7.4% of samples had a biotin concentration at or above 10 ng/mL (considering a low threshold, above which interference will occur for the most sensitive immunoassays) [107]. In Australia, 0.8% (4/490) of patients sampled presented with a biotin concentration above 10 ng/mL, whereas in the Netherlands, this percentage was estimated to be 0.2% [108, 109]. In the UK, no patients presented with a biotin concentration above 2.5 ng/mL in a group of 524 patients examined in 2020 [110].

Recent therapeutic protocols involving very high doses of biotin (300 mg) for progressive multiple sclerosis have highlighted the biotin problem in the last four years [111]. Since the most recent studies (by the end of 2020) showed the ineffectiveness of these very high doses for progressive multiple sclerosis, with a risk of erroneous laboratory results and associated negative consequences, these protocols will now be abandoned [112, 113]. Lastly, hospital departments specialized in the detection of inborn errors of metabolism use biotin in their protocols for several biotin-responsive medical conditions such as biotinidase deficiency, holocarboxylase synthetase deficiency, and biotin-thiamine basal ganglia disease, with high biotin doses being prescribed [102, 114-116]. The biotin-associated risk is relevant in neonatal care, as biotin can be empirically (and temporarily) prescribed for neonatal epileptic encephalopathy [117].

For susceptible methods, the magnitude of error is proportional to the free biotin concentration in the sample; for very high doses of biotin, extreme pathological results may be recorded [118]. The most problematic situations are high doses administered for inborn errors of biotin metabolism, multiple sclerosis, and kidney failure, since biotin is mostly eliminated through the kidneys [99, 101, 119, 120]. With moderately high intake such as 10 mg (for cosmetic purposes), the extent of analytical error is less remarkable as far as endocrine assays are concerned, but these doses remain a main source of confusing erroneous results. The major determinants of such errors for susceptible immunoassays are the biotin dose, time elapsed since last intake, and kidney function if altered. The maximum biotin concentration is observed approximately 1.5 hours after intake, and the half-life of biotin is 15 hours on average [121-124]. The susceptibility of different immunoassays involving streptavidin-biotin separation is also highly variable.

Different strategies have been proposed to minimize the risk associated with biotin for susceptible methods [125, 126]. Each laboratory should evaluate this risk according to methods used and specific recruitement (e.g., inborn errors of metabolism) [90]. The reformulation of immunoassays for biotin-resistant methods is successfully progressing, but many biotin-susceptible methods remain in widespread use [127].

While waiting for these improvements, public education and patient awareness of this issue are necessary. Because of this new situation, a component that can interfere with laboratory assays is continually being absorbed by a significant number of patients. Therefore, inquiry about biotin intake has become a key question. Patients who need laboratory assays should be notified to refrain from taking any supplement and allow several hours or days to “wash out” any residual biotin. Since the washout period needed will vary according to the assay performed, no single recommendation can be given for the time of washout [93, 122].

In patients with inborn errors of metabolism, biotin administration cannot be stopped, and in case of emergencies, it is not possible to wait for hours or days for biotin clearance; therefore, a contingency procedure must be established by the laboratory for these cases if the methods in use are susceptible to biotin interference [118].

Not all laboratories have the capability for biotin measurements, making it difficult to identify supra-physiological biotin intake; dilution tests and neutralization assays can help when suspecting this problem in a patient [120, 128, 129]. Some biotin-sensitive tests have been used as “biotin-detecting tests,” (e.g., false high testosterone measurements in women, false high estradiol measurements in men) [130]. Once biotin interference is identified, it should raise the possibility of other affected results for this patient.

ASAs

ASAs in a patient’s serum can cause the same bidirectional interference as found for biotin (i.e., falsely lowered in sandwich immunoassays and falsely increased in competitive assays). Unlike biotin, this interference is endogenous and is thus suspected to be non-transient. Given the possibility of interference for an extended time, cautioning the patient is necessary to provide information on the potential effect of this Ab on future medical examinations and to avoid the risk of future inappropriate treatments or investigations [131]. The seroprevalence of ASA seems to be higher than previously thought [132, 133]. Interference analysis in samples from 42 patients presenting with discordant thyroid assay results with a streptavidin-biotin methodology, 34 cases were found to be due to ASA [133]. In another study involving an anti-cyclic citrullinated peptide assay, 0.6% of the patients presented with a false-positive result due to the presence of ASA [134]. The mechanism of appearance of this Ab is still not elucidated. Streptavidin is produced by Streptomyces avidinii, a soil microorganism, and the circumstances that could lead to immunization are unknown. Based on the cases reported to date, the interferent will have a more pronounced effect on competitive immunoassays than on sandwich immunoassays; for example, FT3 and FT4 concentrations could be overestimated, whereas the TSH concentration could be apparently lowered, but not fully suppressed, as should be recorded in a real hyperthyroid patient sample. This Ab is less potent than biotin (with extremely high affinity for streptavidin, and higher than any Ag–Ab binding). The lack of TSH suppression, associated with dramatically high “thyroid hormone” concentrations, will be noticed and evoke the syndrome of inappropriate thyrotropin secretion [131, 135-137]. By affecting a common step in immunoassays, as for biotin, multiple erroneous results can be recorded [131, 133, 137, 138].

Interference affecting signal generation or quantification

Rarely, the affected element in the immunoassay is the molecule that is supposed to generate the signal to enable quantification of the analyte. In some patients, an interferent present in vivo will inhibit the production of a measurable signal. For example, interference from the ruthenium signal led the manufacturer to modify and improve the ruthenium label and linker, as well as to add Ab polymers to block anti-ruthenium substances. The interfering factor could be an anti-ruthenium Ab or some unidentified substance [139, 140-143]. The anti-ruthenium component diminishes the amount of signal, resulting in false high or false low analyte concentrations, depending on the assay format. The magnitude of interference in competitive immunoassays (particularly FT4 and FT3) seems to be more important than that in sandwich immunoassays, indicating that the thyroid profile may evoke the syndrome of inappropriate TSH secretion [140, 142, 143]. When the presence of an anti-ruthenium Ab is confirmed, the origin of the immunization is not known. Buijs, et al. [140] proposed that anti-ruthenium Abs might be induced by the intake of ruthenium from the food chain or following exposure to residues on clothing (as ruthenium is used in the dying industry). It is also possible that the immune reaction against ruthenium (or ruthenium binding to the immunoassay reagent) is coincidental.

Other cases of interfering Abs directed against other labels have been sporadically reported in competitive assays using method-specific labels [144, 145]. These include falsely elevated androstenedione concentrations owing to Abs against the horseradish peroxidase label and erroneous estradiol and estriol concentrations due to anti-bovine alkaline phosphatase Abs, which can induce both positive and negative interferences because of the heterogeneity of available epitopes. Synthetic alkaline phosphatase (asfotase alfa) is a pharmacological recombinant alkaline phosphatase that is approved as the first therapy for hypophosphatasia, a rare inherited disease; a patient taking asfotase alfa will show a false low testosterone concentration in alkaline phosphatase-conjugated immunoassays. The proposed mechanism is that elevated phosphatase is not sufficiently removed during the washing step, and a falsely elevated signal will be produced, translating to a false low testosterone concentration because of the competitive design [146]. Fluorescein, used for ophthalmologic angiography examination, can also disturb fluorescent signal measurement in immunoassays involving a fluorescence measurement [147, 148].

Other conditions that affect immunoassays

The presence of particular proteins within the biological sample can disturb Ag–Ab binding and the awaited equilibrium and can induce laboratory test distortion.

Monoclonal gammopathies

“Paraproteins,” specifically monoclonal Igs, can affect Ab binding and cause interference in TSH immunoassays, either by hindering the recognition of the Ag by binding to an idiotope of a reagent Ab or by behaving like a heterophilic Ab [149, 150]. The interference caused by these mAbs can be transient and is method-specific [150, 151]. HBT can efficiently remove these mAbs or can fail to reduce such interference [150-152]. Dilution tests may or may not be efficient in demonstrating the presence of interference [150, 152, 153]. A recent study demonstrated complex interference in some 25-hydroxy (OH) vitamin D immunoassays in eight patients, involving paraproteins (IgG, IgM, or IgA) [154]. An effect of the dissociation agent (added to release 25-OH vitamin D from its binding proteins), leading to precipitation, is evoked in the presence of the monoclonal component. This underlines the complexity of some interfering mechanisms, although simple PEG precipitation was found to be effective in removing the interference. The extent of interference seems to correlate with the concentration of the monoclonal component in some case reports [152, 155].

Binding proteins and free hormone measurements

Free hormone measurements are aimed at avoiding the influence of binding proteins and to obtain a better estimate of hormone actions compared with total hormone measurements. Although free thyroid hormone assay accuracy has been greatly improved in recent decades owing to the improvement in methodologies and tracers, their fragility remains evident for some patient groups such as patients with non-thyroidal illness (NTI), pregnancy, familial dysalbuminemic hyperthyroxinemia (FDH), and those presenting with thyroid hormone Ab (see the anti-analyte Abs section) [156]. The first two conditions (NTI and pregnancy) represent an analytical challenge because of the large, adaptive modifications of binding proteins, and free thyroid hormone estimates in these conditions remain a subject of debate [156]. FDH is a dominantly transmitted condition, in which an albumin variant is present with increased affinity for T4 (approximately 60-fold). This syndrome does not cause disease, is associated with increased circulating total T4 concentrations, and is a source of spuriously elevated FT4 concentrations (possibly associated with elevated FT3 concentrations) [157]. Current free thyroid immunoassays frequently produce artifactual results, although with varying susceptibility, irrespective of a two-step or a one-step design [158, 159]. The prevalence of FDH in the Caucasian population is estimated at 1 in 10,000 patients with the prevalence in patients of Hispanic origin being much higher (1.0–1.8%), whereas this condition was reported to be extremely rare in Japan [160-162]. The R218H albumin variant is the most frequent in FDH, although R218P and R218S can also be detected. FDH can mimic the biochemical picture of inappropriate TSH secretion (whether due to resistance to thyroid hormone or to TSH-secreting pituitary adenoma) and seems to be an underdiagnosed entity; therefore, strategies have been established to avoid this pitfall [163, 164]. FDH can be identified by radiolabeled T4-binding electrophoresis and albumin gene sequencing [157].

Free testosterone concentration measurements are very challenging, and direct methods using an “analogue” tracer are a subject of caution and not widely recommended in clinical guidelines. Equilibrium dialysis and ultrafiltration methods are considered the gold standards to separate the bound form from free hormone. However, these methods are labor-intensive and present many technical issues; further, they lack common reference ranges and are not widely adopted in routine clinical laboratories [165, 166]. Several equations have been proposed to estimate the calculated free testosterone concentration in both men and women [166].

Complement

Negative complement interference can cause an increase in AMH concentrations in stored sera as compared with the results in fresh sera [167]. An interaction between complement fraction C1q and the immobilized anti-AMH capture Ab is followed by activation of the complement cascade pathway, with C3 cleavage and C3b deposition. The steric hindrance from this complex prevents AMH binding to the capture Ab. This assay is particularly susceptible due to the use of the IgG2a isotype as the capture Ab since this Ig has potent complement-activating abilities [168]. This problem is now avoided with the use of EDTA samples or EDTA-containing buffers to pre-dilute the sample, which reduces interference from calcium-modulated complement activation.

CIRCUMSTANCES OF SUSPICION OF INTERFERENCE IN CLINICAL LABORATORIES

Analytical artifacts must be considered in one or more of the following situations [10]: (1) lack of coherence with the clinical presentation and other investigations, such as a thyrotoxic biochemical profile in a clinically euthyroid patient, undetectable FSH/LH in a young patient who has completed puberty with no signs of gonadotrophin deficiency, or normal prolactin in a patient with a known prolactin-secreting tumor [28]; (2) extremely unusual analyte concentrations, even in pathological states; (3) disrupted normal physiological regulatory feedback loops, evoking, for example, the very rare syndrome of inappropriate TSH secretion [163]; (4) inconsistent laboratory results obtained by different analytical methods, since the analytical errors are often method-dependent (notably for the streptavidin–biotin separation methods or signal-specific methods [57, 142]); (5) different results from anterior assays without any possible explanation, such as therapeutic-induced evolution.

Cases in which the results are falsely normal or slightly abnormal, although clinically plausible, are more difficult to detect [30, 51]. Laboratories must pay special attention to certain patient groups (e.g., those with hereditary disorders or autoimmune disorders, and those receiving immunotherapy or neurosurgery). Some external quality assessment schemes have specifically focused on some of the interference types reviewed herein (e.g., macroprolactin, pegvisomant therapy, proopiomelanocortin, HCG hook effect, and biotin) to raise awareness on these problems [5, 95, 169].

SOLUTIONS IN THE FACE OF SUSPECTED INTERFERENCE

When laboratory specialists suspect interference, different approaches are possible. These approaches are general and do not always identify the exact nature of the interfering agent, whereas others are more specific. The first question to answer is: “is there interference?”

Repeating the measurements and then questioning the complete assaying process is the starting step.

Strategies and algorithms have been defined, either in general or dedicated to thyroid function, Tg, or PTH assays [2, 31, 75, 170-172]. The most recent strategies consider the biotin problem [31, 170]. Each laboratory must validate the interference testing protocol for each immunoassay, as some methods are not valid after HBT or PEG pretreatment [173]. Methods involving a second Ab separation step prohibit the use of any blocking agent containing a mouse component [174]. Negative controls (and positive controls if available) are also needed.

A troubleshooting list is proposed in Table 3. This list supposes that method-specific interference or those related to specific situations have been identified, such as biotin treatment or new therapies. A useful approach could be to add a warning of a specific interference to remind clinicians of a possible pitfall or limitation of the assay (e.g., burosumab in the FGF23 analysis report). When possible, a new sample obtained after a washout period will be needed if an exogenous interferent is identified in the therapeutic file of the patient.

Table 3

Troubleshooting the most frequent types of immunoassay interference

Interference type[†]	Error type	Identification	Troubleshooting
Method-specific interference
Biotin	Competitive assay: ↑Sandwich assay: ↓	Patient’s fileAdsorption if validatedDilution	Withdraw biotin if possible, and obtain a new sampleTest with an alternative method
Anti-streptavidin antibody	Competitive assay: ↑Sandwich assay: ↓	Adsorption if validated	Test with an alternative method
Signal-specific antibody interference (anti- ruthenium, anti-alkaline phosphatase)	Competitive assay: ↑Sandwich assay: ↓	Alternative method comparison	Alternative method needed
Fluorescence signal	↑ or ↓	Fluorescein injection	Obtain a new sample after washout
Alkaline phosphatase label	↑ or ↓	Recombinant alkaline phosphatase therapy	Obtain a new sample after washout, if possible
Common interference
Hook effect (prolactin, HCG, Tg, calcitonin)	↓	Progressive dilutions	Two coherent successive dilutions
Cross-reaction	Competitive assay: ↑ Sandwich assay: ↑ or ↓ (depending on specificity characteristics)	Patient’s file, therapeutic information	Appropriate interpretationLC-MS/MS control (steroid assays)
Macro analyte (prolactin, TSH, FSH, LH)	↑	PEG precipitationRecovery testGel filtration chromatography	Appropriate interpretation and percent recovery post-PEG
Anti-insulin Ab (insulin assay)	↑ or normal	Assay anti-insulin Ab
Anti-Tg Ab (TG assay)	↓	Assay anti-Tg	Control TG with LC-MS/MS, if available
Burosumab therapy (intact FGF23 assay)	↓	Patient’s file, therapeutic information	C-terminal FGF23 assay, if available
Heterophile Ab, HAAA, RF (all assays)	Mostly ↑↓ possible	Dilution testHBT pretreatmentPEG pretreatmentRF assayRF adsorbentAdding non-immune IgPatients’ file: looking for immunotherapy, auto-immune context	Alternative method needed
Gammopathy (all assays)	↑↓ possible	Dilution testHBT pretreatmentPEG pretreatmentProtein electrophoresis	Alternative method needed
FDH, thyroid hormone autoantibody (FT4, FT3 assays)	↑	Specific assay	Notify in patient’s file, alternative methods needed

†Interferences are either method-specific or common to all immunoassays (although errors of different magnitudes are recorded among the different methods).

Abbreviations: Ab, antibody; HAAA, human anti-animal antibody; FDH, familial dysalbuminemic hyperthyroxinemia; FGF, fibroblast growth factor; FSH, follicle stimulating hormone; FT4, free thyroxine; FT3, free triiodothyronine; HBT, heterophile blocking tube; LC-MS/MS, liquid chromatography coupled to tandem mass spectrometry; LH, luteotropin hormone; PEG, polyethylene glycol; RF, rheumatoid factor; TSH, thyroid stimulating hormone; Tg, thyroglobulin.

Among the different interference types, cross-reactivity is more or less foreseeable. This is mentioned in the reagent package insert, because cross-reaction from closely related molecules is usually tested by the manufacturer (although cross-reaction might be studied with a single, clinically irrelevant concentration). When a cross-reaction is suspected, appropriate interpretation of the result is helpful. In contrast, the presence of endogenous Abs is unpredictable, sporadic, and may induce complex analytical interference and inaccuracy [153].

Measuring an analyte using another method is very useful and essential, provided that the methodology used is different; this implies that an alternative method is available, for example in nearby laboratories. For steroid immunoassays, liquid chromatography coupled to tandem mass spectrometry (LC-MS/MS) will be the most appropriate control method.

Serial dilution of the sample is the simplest approach when interference is suspected (or for a hook effect). This could be an orienting assay and an adapted diluent must be used. Some immunoassays do not support sample dilution because of the matrix effect or because they “resist” dilution (e.g., free thyroid hormone assays) [175]. When applied, the dilution test will demonstrate negative or positive interference. However, it can be challenging to interpret dilution test results, as some samples with heterophile Abs can give a linear response (falsely confirming the original results) or a nonlinear response (potentially causing false confirmation of suspected interference) [29, 176]. A dilution test introducing animal serum or Ig (from the same species) can be useful [177].

No single test can identify or rule out interference from an endogenous Ab. Identifying Ab interference might involve the use of HBTs (Scantibodies Laboratory, Santee, CA, USA), dilution test, RF-absorbents, PEG precipitation, and protein A and G pre-adsorption or the addition of animal serum or Ig (see Sturgeon [2] for a description of the protocols). The use of three simple tests (dilution test, HBT pretreatment, and PEG precipitation) could identify interference in 90% of suspected samples [153].

Samples from patients with a known history of rheumatoid arthritis or other autoimmune diseases associated with RF presence can help determine the cause of interference. Some commercial assays can detect HAMA‐positive samples [178]. Notably, none of these commercial assays can detect all HAMA clones; thus, negative results based on these assays do not exclude the presence of an interfering HAMA [179].

Biotin interference is method-specific and can be simply overcome by comparing the results with those of a different separation methodology. The neutralization of biotin or ASA can be obtained with the aid of a high-capacity streptavidin solid phase [120, 128, 129, 180]. Other particular approaches are as follows:

- Heterophilic Abs are found in serum, plasma, or whole blood. Such interference is not found in urine; thus, discordant results with urine, for molecules eliminated in the urine, are an excellent way to detect this interference (HCG, cortisol) [177].

- A comparison of results obtained in newborns (e.g., elevated TSH screening result) with those observed in the mother can be helpful [71].

- Simultaneous measurements of procalcitonin can be useful to exclude a falsely elevated calcitonin result due to heterophilic Ab interference [181].

Precise identification of the interferent may require a specialized laboratory. For example, FDH requires a specialized technique using radiolabeled T4 capture by serum protein and albumin gene sequencing. Manufacturers can also help identify an interference.

FUTURE PERSPECTIVES

Improvements in assay design, Ab structure and specificity [196], and signal generation and detection, with an increasing number of assays developed to detect more molecules, have made immunoassays one of the most used techniques in clinical laboratories. However, there has also been a trend to simplify methods to facilitate automation, and new innovative therapies result in new interferences.

Some of the major specificity problems in competitive assays are related to the measurement of steroids and structurally related compounds. Therefore, many laboratories have started using LC-MS/MS for the quantification of these analytes, although these methods are more expensive and technically demanding than immunoassays. LC-MS/MS avoids main specificity problems and also provides multi-parameter quantification in the same analytical session, allowing for steroid profiles to be generated with a dramatically reduced sample volume, which is valuable for newborns and infants. Unfortunately, these powerful and reliable measurements are not yet adapted to high-throughput sandwich assays. As protein and macromolecule assays with LC-MS/MS become more amenable, the use of immunoassay-based measurements may decline to improve specificity and robustness with respect to immunological interference, notably for some critical assays such as Tg as a major biomarker for the follow-up and management of differentiated thyroid cancer [75]. While waiting for these improvements, immunoassays, despite their drawbacks, will still be in general use, at least for a few years, and the problem of immunoassay interference will persist.

Laboratory knowledge plays a central role in highlighting possible interference. When a clinician deals with unexpected or incoherent results regarding patient conditions, a strong interface with laboratory specialists facilitates the rapid identification of incoherent results. Informing the clinical staff of the ever-present possibility of unexpected sporadic interference, notably from an endogenous Ab, is needed [2].

When facing unknown interference, which might require more deep and specialized investigations, feedback from laboratory to manufacturers enables the manufacturers to actively search for a solution to the emerging problem and to keep improving the immunoassay robustness with respect to the risk of interference. Granting laboratory specialists access to the clinical and therapeutic records of patients is important when they suspect and try to detect interference. Specifically, the notion of biotin or a specific therapy has become a key question. In addition, the notion of previously administrated immunotherapies must always draw the attention of laboratory specialists to the possibility of Ab-induced interference in immunoassays. Ideally, an interfering therapy should automatically be flagged; thus, minimizing interference risk can also be achieved by connections between health information systems and laboratory information systems.

CONCLUSION

Immunoassays are inherently fragile but will remain in practice for many hormone measurements for years to come. This review outlines the importance of having excellent knowledge of the design and characteristics of laboratory immunoassays to appropriately suspect interference. Changes in medical practice and development of new therapies and sociological trends (such as biotin-loaded dietary supplements) might affect immunoassay-based diagnoses. New interferents will be identified; therefore, laboratory specialists should not ignore or underestimate immunoassay weaknesses and should establish a bi-directional, open, and permanent dialogue with clinicians to rapidly identify any suspected results before making further diagnostic or therapeutic decisions.