Testosterone - CAM 131HB

Description/Background
Testosterone is a naturally occurring lipophilic androgen hormone that is produced by both males and females for various functions. In males, testosterone is produced by the interstitial cells of Leydig in the testis. In females, testosterone is primarily created and disseminated by the ovaries and adrenal glands. Testosterone is required for synthesis of dihydrotestosterone (DHT) as well as estradiol (E2). Sex hormone-binding globulin (SHBG) binds testosterone to aid in transport and intratesticular bioavailability. 

Dysregulation in testosterone levels can lead to serious conditions, including hypogonadism and other testosterone excess or deficiency conditions. Additional hormones, including follicle-stimulating hormone (FSH), luteinizing hormone (LH), and prolactin, play roles in development. As part of the hypothalamic-pituitary-gonadal axis, FSH and LH bind to gonadal receptors to modulate testosterone. During conditions of dyshomeostasis, such as hypogonadism, FSH, LH, and prolactin serum levels can be used as diagnostic tools (Bhasin et al., 2018; Gill-Sharma, 2018). 

Terms such as male and female are used when necessary to refer to sex assigned at birth.

Policy

  1. Measurement of serum total testosterone (see Note 1) is considered MEDICALLY NECESSARY in any of the following situations:
    1. For symptoms of androgen deficiency or androgen excess in males:
      1. For initial screening, two measurements at least 24 hours apart.
      2. If the initial screening was normal but symptoms persist, follow-up testing is allowed no sooner than 60 days after the initial screening.
    2. For the monitoring of treatment response in men taking enzyme inhibitors for prostate cancer.
    3. For men receiving testosterone replacement therapy (every 2 – 3 months for the first year after initiation of therapy or after a change in therapeutic dosage; annually thereafter).
    4. For gender-dysphoric/gender-incongruent persons (baseline, during treatment, and for therapy monitoring).
    5. For symptomatic females (see Note 2) being evaluated for conditions associated with androgen excess (e.g., polycystic ovary syndrome and functional hypothalamic amenorrhea).
  2. For males with total testosterone confirmed as low or borderline low and who have hypogonadism, gynecomastia, and/or other forms of testicular hypofunction, annual measurement of serum free testosterone, sex hormone-binding globulin (SHBG), and/or albumin is considered MEDICALLY NECESSARY.
  3. For individuals suspected of having a disorder that is accompanied by increased or decreased SHBG levels (see Notes 3 and 4), measurement of serum free testosterone using a medically accepted algorithm based on total serum testosterone, SHBG, and/or albumin or bioavailable testosterone is considered MEDICALLY NECESSARY.
  4. Prior to initiating testosterone therapy for males with gynecomastia, once per lifetime serum estradiol measurement is considered MEDICALLY NECESSARY.
  5. For individuals with ambiguous genitalia, hypospadias, or microphallus, measurement of serum dihydrotestosterone for the diagnosis of 5-alpha reductase deficiency is considered MEDICALLY NECESSARY.
  6. Measurement of serum free testosterone and/or bioavailable testosterone as a primary test (i.e., in the absence of prior serum total testosterone measurement) is considered NOT MEDICALLY NECESSARY.
  7. For asymptomatic individuals or for individuals with non-specific symptoms, measurement of serum total testosterone, free testosterone, and/or bioavailable testosterone is considered NOT MEDICALLY NECESSARY.
  8. For the identification of androgen deficiency in women, measurement of serum testosterone is considered NOT MEDICALLY NECESSARY.

The following does not meet coverage criteria due to a lack of available published scientific literature confirming that the test(s) is/are required and beneficial for the diagnosis and treatment of a patient’s illness.

  1. The use of saliva for the measurement of testosterone is considered NOT MEDICALLY NECESSARY.
  2. For all other situations not mentioned above, measurement of serum dihydrotestosterone is considered NOT MEDICALLY NECESSARY.NOTES:

Note 1: Serum total testosterone sample collection should occur in the early morning, after fasting. Due to considerable variability in serum total testosterone levels, the Centers for Disease Control and Prevention (CDC) developed a standardization program for total testosterone assays (Hormone Standardization [HoSt]/Testosterone). An assay certified by the CDC’s HoSt/Testosterone program is standardized to within ±6.4% of the CDC total testosterone reference standard. It is STRONGLY RECOMMENDED that serum total testosterone measurement be performed with an assay that has been certified by the CDC HoSt/Testosterone program (Bhasin et al., 2018). A list of CDC-certified assays is available on the HoSt website (CDC, 2023).

Note 2: When measuring serum total testosterone in females, please note that the technology used for measurement must be sensitive enough to detect the low serum total testosterone levels that are normally found in females.

Note 3: Conditions associated with decreased SHBG concentrations according to the 2018 Endocrine Society Guidelines (Bhasin et al., 2018):

  • Obesity
  • Diabetes mellitus
  • Use of glucocorticoids, progestins, and androgenic steroids
  • Nephrotic syndrome
  • Hypothyroidism
  • Acromegaly
  • Polymorphisms in the SHBG gene

Note 4: Conditions associated with increased SHBG concentrations according to the 2018 Endocrine Society Guidelines (Bhasin et al., 2018):

  • Aging
  • HIV disease
  • Cirrhosis and hepatitis
  • Hyperthyroidism
  • Use of some anticonvulsants
  • Use of estrogens
  • Polymorphisms in the SHBG gene

Table of Terminology

Term

Definition

AAP

American Academy of Pediatrics

ABIM

American Board of Internal Medicine

ABP

Androgen binding protein

ACOG

The American College of Obstetricians and Gynecologists

ACTH

Adrenocorticotropic hormone

ADT

Androgen deprivation therapy

AFP

Alpha- fetal protein

AIDS

Acquired immunodeficiency syndrome 

AUA

American Urological Association

CBG

Corticosteroid-binding globulin-bound testosterone

CDC

Centers for Disease Control and Prevention

CLIA’88

Clinical Laboratory Improvement Amendments of 1988

CMAJ

 Canadian Medical Association Journal

CMS

Centers for Medicare & Medicaid

CSAM

Canadian Society of Endocrinology and Metabolism

CUA

Canadian Urological Association

CV

Coefficient of variation

DHEAS

Dehydroepianandrosterone sulphate

DHT

Dihydrotestosterone

E2

Estradiol

EAA

European Academy of Andrology

EAU

European Association of Urology

ELISA

Enzyme linked immunosorbent assay

ES

The Endocrine Society

ESI

Electrospray ionization

FDA

Food and Drug Administration

FHA

Functional hypothalamic amenorrhea

FSH

Follicle-stimulating hormone

FT

Free testosterone

Gy

Gray unit of ionizing radiation

hCG

Human chorionic gonadotropin

HIV

Human immunodeficiency Virus

HoSt

Hormone standardization

HPLC

High performance liquid chromatography

ID

Isotope dilution

ID-LC-MS

Isotope dilution-liquid chromatography-tandem mass spectrometry

IGHG

International Late Effects of Childhood Cancer Guideline Harmonization Group

LC-MS/MS

Liquid chromatography-tandem mass spectrometry

LDTs

Laboratory-developed tests

LH

Luteinizing hormone

LOH

Late onset hypogonadism

MRI

Magnetic resonance imaging

MS

Mass spectrometry

NCCN

National Comprehensive Cancer Network

OH

Hydroxy

ORM

Orosomucoid bound testosterone

PADAM

Partial androgen deficiency

PCOS

Polycystic ovary syndrome

PCSF

PanCareSurFup

PRL

Prolactin

PSA

Prostatic specific antigen

SHBG

Sex hormone binding globulin

SHBG

Sex hormone binding globulin bound testosterone

TBI

Traumatic Brain Injury

TBS

Trabecular bone score

TSH

Thyroid stimulating hormone

TT

Total testosterone

vBMD

Volumetric bone mineral density

WC

Waist circumference

Rationale 
The steroid hormone, testosterone, plays a role in both male and female development and health. In males, testosterone is involved in the stage-specific differentiation of germ cells, spermatogenesis, and the synthesis of dihydrotestosterone (DHT) and estradiol (E2). DHT stimulates sexual differentiation of male genitalia during embryogenesis, genital maturation during puberty, and growth of pubic and facial hair (Kinter & Anekar, 2020). E2 is required in males for modulating libido, erectile function, and spermatogenesis (Schulster et al., 2016). Serum testosterone is typically solubilized by binding to the androgen-binding protein (ABP) or sex hormone-binding globulin (SHBG), which aids in regulating their transport, distribution, metabolism, and biological activity. ABP and SHBG have similar primary structure, but they differ in the types of oligosaccharides associated with them (Hammond & Bocchinfuso, 1995).  

In females, testosterone is primarily synthesized and secreted in the ovaries and adrenal glands (Longcope, 1986) but some testosterone production also occurs in peripheral tissues like muscle, fat, breast, and bone (Burger, 2002). Polycystic Ovary Syndrome (PCOS) is one manifestation of a dysregulation of testosterone in women and is a complicated condition with a variety of metabolic, reproductive, and psychological features (Teede et al., 2018).

Primary and secondary hypogonadism are two forms of testicular hypofunction found in males. These conditions can be differentiated by the concentration of serum luteinizing hormone (LH), follicle-stimulating hormone (FSH), and prolactin. Primary hypogonadism is associated with low levels of testosterone and normal to high levels of LH and FSH. Secondary hypogonadism is associated with low levels of testosterone and normal to low levels of LH and FSH (Carnegie, 2004). The anterior pituitary gland of hypothalamic-pituitary-gonadal axis releases LH and FSH, which act on the gonadal receptors to regulate testosterone production. Binding of LH to Leydig cell receptors initiates testosterone production, while testosterone secretion is further regulated by feedback inhibition (Nassar & Leslie, 2023). Males who develop hypogonadism prior to puberty often exhibit depressed secondary sex characteristics, eunuchoid stature, small testes, gynecomastia, and a small phallus. For males who develop hypogonadism after the onset of puberty, the physical findings are similar, except for a normal stature and normal phallus size (Snyder, 2022). Besides hypogonadism, testosterone production can also be affected by certain medications, chemotherapy, lifestyle, and aging (Meldrum et al., 2012; Nassar & Leslie, 2023).

In adult males, total serum testosterone levels decrease at an average rate of 1.6% per year. The concentrations of free and bioavailable testosterone decrease more rapidly, typically two to three percent annually, due to the natural increase in SHBG. By the age of 60, 20% of men will have testosterone levels below the normal range, “and the figure rises to 50% in those aged over 80” (Stanworth & Jones, 2008). Significant decrease in testosterone may result in symptoms such as fatigue, decreased libido, erectile dysfunction, depression, muscle weakness, and others. Unfortunately, these symptoms are not specific to testosterone deficiency (Bhasin et al., 2018). Low testosterone levels are associated with diabetes (Hassanabad & Fatehi, 2018), metabolic syndrome (Mohammed et al., 2018), cardiovascular disease (Corona et al., 2018; Wang et al., 2018), obesity (Molina-Vega et al., 2018), sleep apnea (Viana et al., 2017), and other disorders (Nassar & Leslie, 2023). Additionally, testosterone elevations are associated with serious conditions including tumors, hyperthyroidism, and genetic disorders such as congenital adrenal hyperplasia (Bhasin et al., 2018; Nassar & Leslie, 2023). 

Within the serum, testosterone can be either free (i.e., not bound to a specific protein) or protein-bound. Only one to four percent of circulating testosterone is usually found free. SHBG binds testosterone with a high affinity whereas serum albumin (HSA), corticosteroid-binding globulin (CBG), and orosomucoid binds testosterone with a much lower affinity. “Bioavailable” testosterone refers to the amount of free testosterone and albumin-bound testosterone as indicated in the figure below (Goldman et al., 2017).


  

CDC Hormone Standardization (HoSt) Program — Testosterone
SSerum testosterone testing can measure either total testosterone (TT) concentration, free testosterone, or bioavailable testosterone. Total testosterone can be “measured using radioimmunoassay, immunometric assays, or liquid chromatography–tandem mass spectrometry. Considerable inter-assay and inter-laboratory variability is often found in TT measurements. When 1133 laboratories using 14 different assays measured TT concentrations using the same College of American Pathologists quality control sample from a single hypogonadal man, the measured values ranged from 45 to 365 ng/dL (1.6 to 12.7 nmol/L)” (Bhasin et al., 2018).

The Centers for Disease Control and Prevention (CDC) released their analysis of total testosterone in serum by isotope dilution-liquid chromatography-tandem mass spectrometry (ID-LC-MS/MS) in 2012. As a part of the CDC HoSt Program (CDC Hormone Standardization Program) to certify and calibrate hormone assays, the CDC monitors and validates hormone testing by laboratories and manufacturers. “Calibration is further verified by analyzing serum material with assigned reference values for total testosterone every 6 months and comparing the results obtained against predefined acceptance limit, which is ± 6.4 % from the target value” (CDC, 2012). According to CDC standards, total testosterone using ID/HPLC/MS/MS methodology has a reportable range of 2.5 – 1000 ng/dL or 0.09 – 34.7 nM with a limit of detection of 0.36 ng/dL or 0.012 nM. As for accuracy in terms of “trueness and precision,” the CDC reports that total serum testosterone precision (%CV) ranges from 2.2% to 5.5%.  The following limitation was noted: “This method was tested for total testosterone analysis in human serum and may not be suitable for other specimens such as plasma, whole blood, urine, and/or saliva. The analytical performance parameters need to be reassessed and verified when other specimen matrices are used” (CDC, 2012). A list of the assays certified by the CDC HoSt/Testosterone program can be found on the CDC’s HoSt website (CDC, 2023).

Analytical Validity
A recent study used a liquid chromatography with tandem mass spectrometry (LC-MS-MS) method to assess salivary testosterone, androstenedione, dehydroepiandrosterone, and 17-OH-progesterone. The authors state that the accuracy of this method is “between 83.0 and 106.1% for all analytes” and conclude that this “LC-MS/MS method allowed a sensitive evaluation of androgen salivary levels and represents an optimal technique to explore the relevance of a comprehensive androgen profile as measured in saliva for the study of androgen secretion modulation and activity in physiologic and pathologic states” (Mezzullo et al., 2017). However, another study compared various ELISA-based salivary testosterone assays and noted that “proportional errors between the methods calls [sic] for caution” as one of the four methods yielded no results due to malfunction (Andersson et al., 2017). Another study compared salivary testosterone measurements using immunoassays with those measured by tandem mass spectrometry. The authors conclude that the immunoassay-based methods “tended to inflate estimates of lower testosterone concentrations” (Welker et al., 2016).

Recently, van der Veen et al. (2019) developed and validated a LC-MS/MS method to establish reliable reference intervals in five plasma steroid hormones (progesterone, 17-hydroxyprogesterone, androstenedione, testosterone and dihydrotestosterone); these researchers utilized samples from 280 healthy male and female participants over a four-month period. Women taking oral contraceptive pills were found to have lower levels of 17-OH-progesterone and androstenedione; further, it was identified that hormonal biological variation was typically greater in women compared to men (van der Veen et al., 2019). Final conclusions stated that “The gender-specific determination of the reference intervals, together with the observation that the biological variation demonstrated a high degree of variation, allows interpretation of data on individual and group level for improved biochemical characterization of patients in clinical practice” (van der Veen et al., 2019).

Star-Weinstock and Dey (2019) developed an accurate and sensitive method to measure testosterone in hypogonadal adults and children of both genders; this quantification method utilized electrospray ionization (ESI)-LC-MS/MS and achieved a “sensitivity of one ng/dL from 100 µL sample volume.” The authors note that two highlights of this novel method are that this sample preparation technique “includes simultaneous protein precipitation and derivatization,” and that this total testosterone measurement method was certified by the CDC Hormone Standardization program (Star-Weinstock & Dey, 2019).

Sun et al. (2020) developed and validated an isotope dilution ultra-performance liquid chromatography tandem mass spectrometry method (ID-UPLC-MS/MS) to measure human serum testosterone. This method offers higher accuracy and lower variability than the traditional immunoassays, especially when measuring low testosterone levels in hypogonadism. To assess accuracy of the method, pure testosterone was added to the serum samples and the actual concentrations after two serial liquid-liquid extractions were measured. The actual concentrations were close to the female and male levels, with a recovery rate ranging from 94.32 to 108.6%. Sensitivity, specificity, and precision were also measured and met the performance criteria standards established by Clinical and Laboratory Standards Institute (Lynch, 2016) and the Hormone Standardization Program of the Center for Disease Control (Yun et al., 2012). “Moreover, the [ID-UPLC-MS/MS] method exhibited a good consistency between low and high concentrations of testosterone. In addition, the method required a simple sample preparation and a small sample volume, therefore it may be suitable for routine clinical practice” (Sun et al., 2020).   

The Centers for Disease Control and Prevention (CDC) reviewed testosterone testing in 2014 in a group of 6746 participants of various age groups and both sexes (Vesper et al., 2014). The positive bias identified by steroid analyte testing indicated that the test was measuring additional compounds (and not only the analyte in question).  The authors concluded that “although technologies for steroid hormone measurement have advanced significantly, measurement variability within and across laboratories has not improved accordingly…  Within-assay variability for current assays is generally high, especially at low analyte concentrations” (Vesper et al., 2014).

Testosterone and other hormones (AMH, FSH, LH, free androgen index (FAI), prolactin, estradiol) have been used for the clinical diagnosis of polycystic ovary syndrome (PCOS). In a study completed by Khashchenko et al. (2020), 130 girls with PCOS had the accuracy and specificity of hormonal testing assessed and cutoffs for the most significant hormone indicators of PCOS diagnosis in adolescents were identified. The authors found that “Levels of testosterone > 1.15 nmol/L, androstenedione > 11.45 ng/mL, and LH/FSH ratio > 1.23 also showed high sensitivity of 63.2–78.2% and specificity of 84.4–93.7% in PCOS diagnosis in the studied sample of girls” (Khashchenko et al., 2020). The combined use of either four thresholds (AMH, FAI, testosterone, androstenedione, LH/FSH ratio as previously stated) yielded a diagnostic accuracy of 90.2-91.6% in predicting PCOS in adolescents (Khashchenko et al., 2020).

Clinical Utility and Validity 
Equilibrium dialysis is the gold standard for determining free serum testosterone. Unfortunately, it is technically difficult and has limited availability. Compared to other less accurate methods, it is expensive. It relies on the accuracy and precision of total testosterone determination. In equilibrium dialysis, a semipermeable membrane is used to retain the bound testosterone on one side of the membrane while the free testosterone equilibrates between the two sides. It is dependent on environmental conditions including pH, ionic strength, and temperature; in fact, steroids, such as testosterone, can bind up to 2.5 times higher at 4◦C than at 37◦C. One study shows that increasing the temperature from 37◦C to 41◦C increased the free cortisol level by approximately 80% (Goldman et al., 2017).  

Immunoassays to measure free and bioavailable testosterone are inaccurate. The Endocrine Society urges the use of medically accepted algorithms that rely on TT, SHBG, and/or albumin to estimate serum free testosterone (Bhasin et al., 2018). Multiple algorithms have been published (Sartorius et al., 2009; Vermeulen et al., 1999; Zakharov et al., 2015). The recent allosteric model proposed by Zakharov and colleagues models the binding of testosterone as a multi-step, dimeric process. This allosteric model has “close correspondence with those measured using equilibrium dialysis” (Zakharov et al., 2015).

A 2017 international study comprised of multiple cohorts with healthy, non-obese males attempted to “derive standardized, age-specific reference ranges” for circulating testosterone; it was stated that “a substantial proportion of intercohort variation in testosterone levels is due to assay differences” (Travison et al., 2017). Further, the issue in developing standards for circulating testosterone due to variation in body mass and comorbidities was also noted. “Another unresolved issue relates to whether the reference sample should include only the healthy nonobese men or whether it should include the entire population of men 19 to 39 years. Obesity and comorbid conditions affect circulating total testosterone concentrations; therefore, inclusion of obese men with comorbid conditions could distort the reference ranges. Whether the reference ranges generated in nonobese men are appropriate for use in obese men deserves further investigation. Even though men with known diagnoses of conditions or diseases associated with hypogonadism were excluded, it is possible a small percentage of individuals in these cohorts may be hypogonadal” (Travison et al., 2017).

Shukla et al. (2018) organized a cross-sectional study to measure the relationship between prostatic specific antigen (PSA) and serum testosterone levels in both healthy men and men with partial androgen deficiency (PADAM); a total of 255 men participated in this study. “Mean total testosterone and serum PSA was 9.35 ± 1.33 nmol/L, 1.96 ± 0.76 ng/mL in males with PADAM and 15.30 ± 1.95 nmol/L, 1.85 ± 0.73 ng/mL respectively in males without PADAM. No significant relationship was observed between serum PSA and serum testosterone levels among healthy males irrespective of PADAM” (Shukla et al., 2018). Results from this study suggest that PSA values do not need to be adjusted “for biopsy decisions according to testosterone levels” (Shukla et al., 2018).

In a retrospective cohort study, eighty-five severely hypogonadal men were observed for changes in serum prostate specific antigen (PSA) concentrations during testosterone treatment for 18 months. The Endocrine Society clinical guidelines recommend measuring PSA in hypogonadal men over the age of 50 at three months and twelve months after starting testosterone therapy and urologic referral if serum PSA > 1.4 ng/mL above baseline or to an absolute value > four ng/mL (Bhasin et al., 2018). Studies have been performed in men with mild to moderate hypogonadism which reported smaller increases in serum PSA concentrations during testosterone treatment; however, no studies have reported serum PSA changes in response to testosterone treatment of severely hypogonadal men. In this study, testosterone treatment “increased the median serum testosterone concentration from 36 ng/dL at baseline to 395 ng/dL at 6-18 months. This treatment resulted in a median increment in PSA above baseline of 0.70 ng/mL at 6-18 months…31% of men had increases in PSA >1.4 ng/mL; and 13% of men reached absolute PSA concentrations > four ng/mL” (Sachdev et al., 2020). The authors suggest that “testosterone treatment of severely hypogonadal men often increases PSA above the commonly accepted thresholds for urologic referral [and] that future clinical guidelines for the expected PSA response to testosterone replacement reflect the degree of hypogonadism” (Sachdev et al., 2020). 

A total of nine years of registry data, comprised of 650 patients with hypogonadism, was analyzed to determine the impact of long-term intramuscular testosterone treatment (1000 mg every 10-12 weeks) (Zitzmann et al., 2019). Serum testosterone concentrations were found to increase “from 5.7±2.3 nmol/L to 19.4±2.8 nmol/L in men with classical hypogonadism and from 7.8±2.4 nmol/L to 19.2±3.1 nmol/L in men with functional hypogonadism”; final conclusions suggest that patients with the functional form of hypogonadism may benefit the most from testosterone treatment as “men with functional hypogonadism were more likely to lose ten percent weight and five percent of waist circumference (WC) than men with classical hypogonadism” (Zitzmann et al., 2019). Men with functional hypogonadism were also more likely to be obese at the start of the study.

Cauley et al. (2021) performed a study to examine the effect of testosterone treatment on TBS. “Two hundred and eleven men were enrolled in Bone Trial of the Testosterone Trials. Of these, 197 men had two repeat TBS and vBMD measurements; 105 men were allocated to receive testosterone, and 92 men to placebo for one year. TBS, a BMD, and vBMD were assessed at baseline and month 12.” The results of this study report that there was no difference in the percent change in TBS by randomized group. They saw a 1.6% (95% confidence intervals (CI) 0.2–3.9) change in the testosterone group and a 1.4% (95% CI−0.2, 3.1) change in the placebo group. In contrast, they saw a six percent increase in vBMD (95% CI4.5–7.5) in the testosterone group as compared to only a 0.4% vBMD change (95% CI−1.65–0.88) in the placebo groups (Cauley et al., 2021). As a result, the authors concluded that TBS was not clinically useful in monitoring the one year effect of testosterone treatment on the bone structure in older hypogonadal men (Cauley et al., 2021).

The Endocrine Society (ES)-Androgen Deficiency Testosterone Therapy 
The ES, in updated 2018 guidelines concerning testosterone therapy and hypogonadism in males, summarized their recommendations with respect to testosterone testing with the following:

  • Recommendation 1.1: “We recommend diagnosing hypogonadism in men with symptoms and signs of testosterone deficiency and unequivocally and consistently low serum total testosterone and/or free testosterone concentrations (when indicated).” (Level 1+++)
  • Recommendation 1.2: “We recommend against routine screening of men in the general population for hypogonadism.” (Level 1++)
  • Recommendation 1.3: “In men who have hypogonadism, we recommend distinguishing between primary (testicular) and secondary (pituitary–hypothalamic) hypogonadism by measuring serum luteinizing hormone and follicle-stimulating hormone concentrations.” (Level 1+++)
  • Recommendation 1.4: “In men with hypogonadism, we suggest further evaluation to identify the etiology of hypothalamic, pituitary, and/or testicular dysfunction.” (Level 2++)
  • Recommendation 3.1: “In hypogonadal men who have started testosterone therapy, we recommend evaluating the patient after treatment initiation to assess whether the patient has responded to treatment, is suffering any adverse effects, and is complying with the treatment regimen.” (Ungraded Good Practice Statement)

Within the explanations and technical comments of the recommendations, the ES specifically states, “Clinicians should not use direct analog-based free testosterone immunoassays, as they are inaccurate.” Moreover, recommendations state that serum total testosterone testing is preferred and should be performed on two separate days after fasting since testosterone concentrations can vary due to many circumstances. For men who initially test low total testosterone, who test near the lower limit, or who have conditions associated with altering sex hormone-binding globulin (SHBG), then free testosterone can be measured either by using an accepted algorithm based on the total testosterone, SHBG, and albumin concentrations or by direct equilibrium dialysis methods rather than the use of immunoassays. As for bioavailable testosterone testing, the ES states, “Measuring bioavailable [testosterone] concentrations using ammonium sulfate precipitation is technically challenging. Furthermore, there are no detailed studies (similar to those described previously that relate FT [free testosterone] concentrations to manifestations of [testosterone] deficiency) that use bioavailable [testosterone] concentrations.” Men beginning hormone replacement therapy should have their serum testosterone and hematocrit levels measured initially to establish a baseline and then, depending on the therapy, have the levels measured again three-to-six months later. While on testosterone therapy, the total testosterone and hematocrit levels should be checked annually thereafter. Concerning secondary hypogonadism, serum prolactin and either serum ferritin or iron saturation measurements are recommended to check for the possibility of reversibility of the condition. The testing algorithm also recommends testing serum luteinizing hormone (LH) and follicle-stimulating hormone (FSH) to differentiate primary and secondary hypogonadism. The algorithm for testing for hypogonadism is shown in the figure below (Bhasin et al., 2018):

The Endocrine Society — Functional Hypothalamic Amenorrhea: An Endocrine Society Clinical Practice Guideline 
TTestosterone testing in addition to other endocrine laboratory tests is recommended as part of an initial endocrine assessment for women with clinical hyperandrogenism in the evaluation of suspected Functional Hypothalamic Amenorrhea (FHA). Functional Hypothalamic Amenorrhea is a condition of anovulation, in which the ovary fails to release an egg during the menstrual cycle and has been correlated with stress, weight loss, and excessive exercise (Gordon et al., 2017). 

The Endocrine Society (ES) - Polycystic Ovary Syndrome (PCOS)
Relative to the diagnosis of PCOS, the ES identifies three criteria that may be evaluated: androgen excess, ovulatory dysfunction, and polycystic ovaries. Two of the three criteria are sufficient for diagnosis, and if both clinical criteria are met, they do not recommend testing for androgen excess. Androgen excess is characterized by elevated serum androgen levels such as elevated total, bioavailable, or free serum testosterone levels. Considering that serum testosterone levels are variable and there is poor standardization of assays, the Task Force recommends familiarity with local assays and does not define an absolute level that is diagnostic of PCOS or other causes of hyperandrogenism (Legro et al., 2013).

The American College of Obstetricians and Gynecologists
In 2018, the ACOG released guidelines on the clinical management of polycystic ovary syndrome (PCOS). In its suggested evaluation of patients with PCOS, the ACOG recommends having a physical, laboratory testing, and an ultrasound examination to confirm the polycystic ovaries. With regards to hormone testing, it includes “documentation of biochemical hyperandrogenemia” by “total testosterone and sex-hormone binding globulin or bioavailable and free testosterone,” but notes to conduct testing that would exclude other causes of hyperandrogenism, such as thyroid dysfunction and hyperprolactinemia. ACOG includes TSH, prolactin, and 17-hydroxyprogesterone as hormones to measure to exclude other causes. The ACOG (2018b) also acknowledges that “there is no standardized testosterone assay in the United States and the sensitivity and reliability in the female ranges are often poor.”

Regarding Müllerian Agenesis, ACOG writes that the initial evaluation of a patient without a uterus “may include the following laboratory tests: testosterone level, FSH level, and karyotype” (ACOG, 2018a).

In 2019, ACOG released a guideline regarding the “screening and management of the hyperandrogenic adolescent.” In it, they state that the diagnosis of hyperandrogenism can be based on clinical symptoms or measurement of serum androgens. However, they recommend against monitoring serum androgens. This guideline was reaffirmed in 2020.

The ACOG recommends identifying clinical symptoms of androgen excess during the initial evaluation. In the proposed algorithm for evaluation, ACOG recommends two separate batteries of hormone tests depending on type of menses. For regular menses, ACOG lists free and total testosterone, DHEAS (dehydroepianandrosterone sulphate), and 17OHP (17-α-hydroxyprogesterone) as hormones that may be tested. For irregular menses, ACOG lists prolactin, LH, FSH, TSH, and the three previously mentioned hormones. ACOG also notes that PCOS may be one of the diagnoses if both androgen excess and irregular menses are identified (ACOG, 2019).

American Urological Association (AUA) 
The AUA published guidelines concerning the evaluation and management of testosterone deficiency in 2018. Five recommendations are given concerning the diagnosis of testosterone deficiency:

  1. “Clinicians should use a total testosterone level below 300 ng/dL as a reasonable cut-off in support of the diagnosis of low testosterone. (Moderate Recommendation; Evidence Level: Grade B)
  2. The diagnosis of low testosterone should be made only after two total testosterone measurements are taken on separate occasions with both conducted in an early morning fashion. (Strong Recommendation; Evidence Level: Grade A)
  3. The clinical diagnosis of testosterone deficiency is only made when patients have low total testosterone levels combined with symptoms and/or signs. (Moderate Recommendation; Evidence Level: Grade B)
  4. Clinicians should consider measuring total testosterone in patients with a history of unexplained anemia, bone density loss, diabetes, exposure to chemotherapy, exposure to testicular radiation, HIV/AIDS, chronic narcotic use, male infertility, pituitary dysfunction, and chronic corticosteroid use even in the absence of symptoms or signs associated with testosterone deficiency. (Moderate Recommendation; Evidence Level: Grade B)
  5. The use of validated questionnaires is not currently recommended to either define which patients are candidates for testosterone therapy or to monitor symptom response in patients on testosterone therapy. (Conditional Recommendation; Evidence Level: Grade C)” 

Other recommendations by the AUA concerning adjunctive testing in males include the following:

  1. In patients with low testosterone, clinicians should measure serum luteinizing hormone levels (Strong Recommendation; Evidence Level: Grade A)
  2. Serum prolactin levels should be measured in patients with low testosterone levels combined with low or low/normal luteinizing hormone levels (Strong Recommendation; Evidence Level: Grade A)
  3. Patients with persistently high prolactin levels of unknown etiology should undergo evaluation for endocrine disorders (Strong Recommendation; Evidence Level: Grade A)
  4. Serum estradiol should be measured in testosterone deficient patients who present with breast symptoms or gynecomastia prior to the commencement of testosterone therapy. (Expert Opinion)
  5. For men undergoing testosterone therapy, “testosterone levels should be measured every 6-12 months while on testosterone therapy. (Expert Opinion)” (Mulhall et al., 2018)

The Endocrine Society (ES)-Endocrine Treatment of Gender-Dysphoric/Gender-Incongruent Persons 
The ES published guidelines suggesting that testosterone level monitoring is suggested at baseline and every 6-12 months during suppression of puberty treatment protocol in gender-dysphoric/gender-incongruent persons. The laboratory monitoring of testosterone levels is also suggested at baseline and every 6-12 months during induction of puberty protocol. Measurement of serum testosterone levels is suggested every three months until levels are in the normal physiologic male range during the monitoring of transgender males on gender-affirming hormone therapy. Testosterone testing is also needed midway between injections for monitoring of testosterone enanthate/cypionate injections, alternatively peak and trough levels could be measured to ensure levels remain in the normal male range. For parenteral testosterone undecanoate, testosterone should be measured just before the following injection. For transdermal testosterone, the testosterone level can be measured no sooner than after one week of daily application (at least 2h after application). For monitoring transgender females on gender-affirming hormone therapy, measurement of serum testosterone is indicated every three months (Hembree et al., 2017). 

American Academy of Pediatrics (AAP) —Choosing Wisely Initiative 
As a part of the Five Things Physicians and Patients Should Question series of the Choosing Wisely initiative of the American Board of Internal Medicine (ABIM) foundation, the AAP states the following: “Avoid ordering LH and FSH and either estradiol or testosterone for children with pubic hair and/or body odor but no other signs of puberty. Premature adrenarche is usually the diagnosis and does not involve activation of the pituitary- gonadal axis but is due to an early increase in adrenal androgens. DHEA-S levels are elevated for age but do not alter the management of this common and generally benign condition” (AAP, 2017).

European Academy of Andrology (EAA) 
The EAA published guidelines concerning management of bone health in males and testing in Andrology, a journal jointly published by the EAA and the American Society of Andrology. Recommendations include the following:

  • “We recommend having serum total testosterone measured twice on a morning blood sample.” (Level 1+++)
  • “We recommend measuring again total testosterone and SHBG if only a single measurement documenting low testosterone is available. LH and prolactin are useful to better characterize hypogonadism.” (Level 1+++)
  • “We do not recommend routine measurement of serum estradiol.” (Level 1++)
  • “We suggest measuring estradiol only when a validated mass spectrometry-based method is available and in rare cases in which severe estrogen deficiency is suspected.” (Level 2++)

Within the evidence and rationale behind the recommendations, the EAA goes on to state, “We suggest using calculated free testosterone when needed, based on the measurement of total serum testosterone, SHBG, and albumin... It can easily be obtained using online available calculators (see Appendix 2 [of (Rochira et al., 2018)] for Web links). Commercially available kits for direct measurement of free testosterone should not be used due to their poor accuracy and reliability” (Rochira et al., 2018). Concerning other hormones, the EEA states, “all patients with documented low serum testosterone consulting with hypogonadal symptoms should receive a biochemical evaluation of their gonadal status, with measurement of serum total testosterone, SHBG, luteinizing hormone (LH), follicle-stimulating hormone (FSH), and prolactin” (Rochira et al., 2018).

The EAA also published clinical practice guidelines regarding gynecomastia evaluation and management. The EAA recommended testing several hormones for gynecomastia including “testosterone (T), estradiol (E2), sex hormone-binding globulin (SHBG), luteinizing hormone (LH), follicular stimulating hormone (FSH), thyroid stimulating hormone (TSH), prolactin, human chorionic gonadotropin (hCG), alpha-fetal protein (AFP), liver and renal function tests” (Kanakis et al., 2019).

The EAA recently published clinical practice guidelines on investigation, treatment, and monitoring of functional hypogonadism in males to provide certain recommendations: 

  1. “We recommend against universal screening for hypogonadism in middle-aged or older men, by structured interviews or questionnaires and/or random total T measurements.
  2. We recommend that the clinical diagnosis of functional hypogonadism should be confirmed by measurement of serum total T with a well validated assay on fasting morning (before 11 am) blood samples obtained on two different days.
  3. Functional hypogonadism should be diagnosed only after exclusion of organic causes of hypogonadism. In addition, to morning total T, luteinizing hormone (LH) should be measured in all patients with suspected functional hypogonadism to differentiate between the primary and secondary causes.
  4. We recommend either measuring or calculating free T (fT), in addition to total T, in patients with conditions that alter sex hormone-binding globulin (SHBG) and when total T concentrations are in the borderline range (~8-12 nmol/L) if the clinical suspicion of hypogonadism is strong” (Corona et al., 2020). 

Above, is a proposed flow chart to diagnose and manage functional hypogonadism (Corona et al., 2020). 

Canadian Urological Association (CUA) and Canadian Society of Endocrinology and Metabolism (CSAM) 
The CUA and CSAM endorsed joint guidelines published in the CMAJ in 2015. The following recommendations were given concerning hormone testing in males for testosterone deficiency syndrome:

  • “We recommend a thorough history and physical examination, instead of the exclusive reliance on standard questionnaires, to identify patients requiring biochemical testing (strong recommendation; moderate-quality evidence).”
  • “The initial biochemical test should be total testosterone level measured in serum samples taken in the morning; determinations of bioavailable testosterone or free testosterone should be restricted to patients with equivocally low total testosterone levels (strong recommendation; high-quality evidence).”
  • “We recommend that sample collection for testosterone measurement occur between seven am and eleven am, or within three hours after waking in the case of shift workers (strong recommendation; moderate-quality evidence).”
  • “Testosterone levels should be measured with the use of testosterone assays traceable to internationally recognized standardized reference material; commercial assays should be certified by the testosterone standardization program of the US Centers for Disease Control and Prevention (strong recommendation; high-quality evidence).”
  • “Measurement of sex hormone–binding globulin with calculated free or bioavailable testosterone should be restricted to men with symptoms of testosterone deficiency and equivocally low testosterone levels (strong recommendation; moderate-quality evidence).”
  • “We recommend investigation for secondary or reversible causes of hypogonadism in all men with testosterone deficiency syndrome (strong recommendation; moderate-quality evidence).”
  • “We recommend investigation for testosterone deficiency syndrome and treatment with testosterone in men with anemia or sarcopenia of undetermined origin (strong recommendation; moderate-quality evidence).”
  • “We recommend assessment of response and adverse effects at three and six months after onset of therapy (strong recommendation; high-quality evidence).”
  • “Testosterone levels should be assessed at three and six months after onset of therapy and then annually thereafter if stable (weak recommendation; low-quality evidence).”

European Association of Urology (EAU) 
In the 2014 EAU guidelines concerning the treatment of castration-resistant prostate cancer, the EAU states, “Follow-up after ADT should include analysis of PSA and testosterone levels, and screening for cardiovascular disease and metabolic syndrome” (Heidenreich et al., 2014).

The European Association of Urology (EAU) recently released guidelines on sexual and reproductive health and expressed the following recommendations for diagnosis of hypogonadism:

  1. “Check for concomitant diseases, drugs and substances that can interfere with testosterone production/action.
  2. Total testosterone must be measured in the morning (7.00 and 11.00 hours) and in the fasting state, with a reliable method.
  3. Repeat total testosterone on at least two separate occasions when below 12 nmol/L and before starting testosterone therapy.
  4. Twelve nmol/L total testosterone (3.5 ng/mL) represents a reliable threshold to diagnose late onset hypogonadism (LOH).
  5. Consider sex hormone-binding globulin and free-testosterone calculation when indicated.
  6. Calculated free-testosterone < 225 pmol/L has been suggested as a possible cut off for diagnosis of LOH. 
  7. Analyse luteinising hormone and follicle-stimulating hormone serum levels to differentiate between primary hypogonadism and secondary hypogonadism forms.
  8. Consider prolactin (PRL) measurement if low desire (or other suggestive signs/symptoms) and low or low-normal testosterone is present.
  9. Perform pituitary magnetic resonance imaging (MRI) in secondary hypogonadism, with elevated PRL or specific symptoms of a pituitary mass and/or presence of other anterior pituitary hormone deficiencies.
  10. Perform pituitary MRI in secondary severe hypogonadism (total testosterone < six nmol/L).
  11. Screen for late onset hypogonadism (including in T2DM) only in symptomatic men.
  12. Do not use structured interviews and self-reported questionnaires for systematic screening for LOH as they have low specificity” (A. Salonia (Chair), 2022). 

The EAU recommends that the standard and most accurate method for testosterone serum testing is Liquid Chromatography-Tandem Mass Spectrometry (LC-MS/MS). Standardized automated platform immuno-assays are reliable techniques to measure testosterone; however, only LC-MS/MS can provide an accurate measurement of free testosterone (fT) levels. There is uncertainty as to what threshold of fT level indicates hypogonadism, but some data indicates that fT levels below 225 pmol/L is associated with hypogonadism. A flow chart for diagnostic evaluation of late-onset hypogonadism is provided below (A. Salonia (Chair), 2022):

National Comprehensive Cancer Network 
Within the algorithm concerning the systemic therapy for castration-naïve disease, the NCCN says to “document castrate level of testosterone if clinically indicated” when assessing progression along with the physical exam and PSA every three to six months. The NCCN also states to “continue ADT [androgen deprivation therapy] to maintain castrate serum levels of testosterone (<50 ng/dL).” Additional recommendations state, “close monitoring of PSA and testosterone levels and possibly imaging is required when using intermittent ADT, especially during off-treatment periods, and patients may need to switch to continuous ADT upon signs of disease progression” (NCCN, 2023b).

The NCCN also published some guidance regarding assessment of hormones for neuroendocrine and adrenal tumors. For pituitary tumors, they list serum prolactin and LH/FSH; for “suspected or confirmed adrenocortical carcinoma”, they list "adrenal androgens (DHEAS, androstenedione, testosterone, 17-hydroxyprogesterone)”; for hypercortisolemic Cushing’s Syndrome, they list ACTH [adrenocorticotropic hormone] (NCCN, 2023a).

International Late Effects of Childhood Cancer Guideline Harmonization Group (IGHG) & PanCareSurFup (PCSF) Consortium 
Within the guidelines and recommendations issued in 2017 by the IGHG and the PCSF Consortium for patients with possible impaired spermatogenesis, it is recommend that “Clinical measurement of testicular volume and of follicle-stimulating hormone and inhibin B might be reasonable for the identification of impaired spermatogenesis in survivors treated with potentially gonadotoxic chemotherapy or radiotherapy potentially exposing the testes in whom semen analysis has been declined or is not possible and who desire assessment about possible future fertility. Be aware of the diagnostic limitations of these tests that may result in false positives or false negatives (level B evidence).” With respect to patients with possible testosterone deficiency, “Measurement of testosterone concentration in an early morning blood sample at clinically appropriate intervals is reasonable in post pubertal survivors treated with radiotherapy potentially exposing the testes to 12 Gy or more or with TBI (expert opinion). In the presence of clinical signs of hypogonadism, or of previous low-normal or borderline testosterone concentrations, or if it is not possible to obtain an early morning blood sample, it is reasonable to measure luteinising hormone concentration in addition to testosterone (expert opinion)” (Skinner et al., 2017).

References 

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Coding Section 

Codes Number Description
CPT  82642 (effective 01/01/2019) Dihydrotestosterone (DHT) 
  82681 (effective 01/01/2021) Estradiol; free, direct measurement (e.g., equilibrium dialysis) 
  84402 Testosterone; free
  84403 Testosterone; total 
  84410 (effective 1/1/2017)  bioavailable, direct measurement (e.g., differential precipitation)
ICD-10-CM  E28.1 Androgen excess 
  E29.0-E29.9 Testicular dysfunction 
  E30.0 Delayed puberty 
  F32.0-F33.9

Depression 

  G47.8-G47.9 Sleep disorders 
  N50.0 Atrophy of testis 
  N50.8 Other spec disorders, male genital organs 
  N50.9 Disorder of male genital organs, unspecified 
  N64.4 Breast pain 
  R41.840 Attention/concentration deficit 
  R41.9 Unspecified symptoms/signs involving cognitive functions and awareness 
  R53.81, R53.83

Fatigue 

  R68.82 Decreased libido 
  Z92.240-Z92.241 Personal history, steroid therapy 
  L70.0-L70.9 Acne 
  R63.5 Excessive weight gain 
  L68.0 Hirsutism 
  N91.0-N91.5 Absent, scanty and rare menstruation 
  N92.0-N92.6 Excessive, frequent/irregular menstruation 
  N94.89-N94.9 Specified conditions associated with female genital organs and menstrual cycle 
  N97.0-N97.9 Female infertility 
  E88.81 Metabolic syndrome (insulin resistance) 
  R73.01-R73.09 Abnormal glucose 
  E08-E13 Diabetes 
  E28.2 Polycystic Ovarian Syndrome 
  E24.0-E24.9 Cushing’s Syndrome 
  E03.9 Hypothyroidism 
  E22.0 Acromegaly 
  E05.0-E05.9 Thyrotoxicosis 

Procedure and diagnosis codes on Medical Policy documents are included only as a general reference tool for each policy. They may not be all-inclusive

This medical policy was developed through consideration of peer-reviewed medical literature generally recognized by the relevant medical community, U.S. FDA approval status, nationally accepted standards of medical practice and accepted standards of medical practice in this community, Blue Cross Blue Shield Association technology assessment program (TEC) and other non-affiliated technology evaluation centers, reference to federal regulations, other plan medical policies and accredited national guidelines.

"Current Procedural Terminology© American Medical Association. All Rights Reserved" 

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