What to Measure: Testosterone or Free Testosterone?

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What to Measure: Testosterone or Free Testosterone? (2021)
Christina Wang and Ronald Swerdloff


1.1 Why Serum Testosterone Is Necessary for the Diagnosis of Testosterone Deficiency?

Low serum testosterone (T) levels in adult men can lead to significant clinical symptoms and signs of testosterone deficiency (TD). These include sexual dysfunction, low energy, and vitality, mood changes, sleep disturbances, loss of body hair, loss of muscle and bone mass, increased visceral fat, mild anemia, and, in more severe testosterone deficiency, small testes and infertility. In adolescent boys, TD presents as delayed sexual development, absence of axillary, pubic, and facial hair, failure of the testes to increase in size, gynecomastia, and eunuchoidal proportions. The symptoms of testosterone deficiency are non-specific, and physical signs may not be clinically detectable in some older men with TD.

In addition, screening questionnaires to assess the symptoms of TD may be useful in large clinical studies; however, they have low specificity and are generally not useful in a clinic to diagnose an individual with TD [1–6]. Even with the use of screening questionnaires and symptoms of TD, the confirmation of TD must be based on the precise and accurate measurement of serum T concentrations [7, 8]. Because serum T can be transiently suppressed during acute illnesses, physical and mental stress, and intensive exercise, T should not be measured when these conditions are present. More importantly, T concentrations may decrease with obesity, age, metabolic syndrome, diabetes, sleep disorders, eating disorders, chronic kidney and liver disease, and chronic use of opiates and glucocorticoids (Table 1.1) [9–14]. Thus, it is important to ascertain the general health of the patient as treatment of some of these conditions may restore serum T to the reference range.



Table 1.1 Common conditions that may affect serum testosterone concentration
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1.2 What Methods Should Be Used for Serum Testosterone Measurements?

Immunoassays are used for measuring serum testosterone concentrations. Several publications in the early 2000s demonstrated that immunoassays used in many clinical laboratories with automated platforms depend on reagents and reference ranges provided by the manufacturers. Some of these automated platform assays provide results that are precise but not accurate with significant bias when compared to the “gold standard” of steroid assays – liquid chromatography-tandem mass spectrometry (LC-MS/MS) [15–17]. These tests had passing scores in proficiency testing when compared to the same method but differed significantly when compared against each other. The T measurements at low concentrations, e.g., in women and children, were most unreliable, which led the Endocrine Society to issue a position statement that emphasized the following : (1) mass spectrometry has better accuracy and specificity and may be the method of choice for measuring testosterone concentrations at low levels; (2) the clinician should know the method and the reference ranges of their laboratories [18]; and (3) standardization programs focusing on accuracy should be implemented and updated reference ranges be established for men, women, and children [18–20]. The Center for Disease Control and Prevention (CDC) Laboratory Science Division took up this challenge and established the Hormone Standardization Program with T measurement as the first hormone to have harmonized assays [21–23]. The goal of the program is not to define which method a laboratory should use but create “testosterone measurements traceable to one accuracy basis allowing measurements to be comparable across methods, time and location” [22]. To date, not only reference and research laboratories participate in the program but also manufacturers of automated platforms and mass spectrometers. The CDC also assisted the College of American Pathology (CAP) to introduce an accuracy-based proficiency test for T assays with the participation of many clinical laboratories [24]. The results of the accuracy-based harmonization of T assays showed that with time (3.5 years) there was an improvement in proficiency scores of both accuracy and precision in 65 participating clinical laboratories in the State of New York [25]. The conclusion is that most clinical laboratories using automated platforms are aware that accuracy-based proficiency testing should be implemented with improvement in the quality of the assay. The accuracy-based tests in the recent CAP report showed very small differences within a method and between methods (Table 1.2). For the diagnosis and monitoring of T-replacement therapy in TD men, both immunoassay and LC-MS/MS methods are sufficient as the goal is to distinguish low concentrations from the population reference ranges of adult men. As shown in Table 1.2, with participation in accuracy-based external quality control, even low levels of testosterone showed good agreement within a method and between methods.


Table 1.2 Accuracy-based testing of serum testosterone (ng/dL) from the College of American Pathologists 2020
1652452870878.png





1.3 What Is the Reference Range for Serum Total Testosterone in Adult Men?

The generally accepted range of serum testosterone in adult men is 300–1000 ng/dL (10.4–34.7 nmol/L) based on immunoassays with a purification step before immunoassays [26]. There are many possible physiological explanations why men would have such a large range of testosterone levels. Once a standardized method has been validated [22], reference ranges can be established based on cross-calibrating assays to a reference method. Using data from four population-based studies in Europe and the United States (1656 younger community-dwelling men in the Framingham Heart Study; European Male Aging Study; Osteoporotic Fractures in Men Study; and Male Sibling Study of Osteoporosis), the harmonized serum testosterone reference range (2.5th to 97.5th percentile) for non-obese men between 19 and 39 years was established to be between 264 and 916 ng/dL (9.16 to 31.8 nmol/L) [27]. Most of these men identified themselves as white and it should be noted that geographical and ethnic/racial differences in sex hormone levels have been reported in some studies [28–30]. Population-based studies of harmonized T levels in other ethnic/racial groups have not yet been reported.




1.4 What Are the Precautions to Reduce the Variability in Serum Testosterone Concentrations?

Serum T concentrations should be measured from a blood sample collected early in the morning between 7 am and 10 am. The diurnal variation of serum T results in T levels higher in the early morning than later in the day in both young and middle-aged men [31]. This diurnal variation is attenuated in older men [32]. Most laboratories establish reference ranges for healthy adult men based on morning samples. Thus, to compare a patient with possible TD, blood samples should be drawn in the morning between 7 am and 10 am. There are data showing that acute ingestion of glucose lowers serum total testosterone by 25% [33]. Thus, for the diagnosis of TD, it is important to obtain a fasting morning blood sample. In general, serum samples should be used for assays. Because T concentrations are affected by acute illnesses, mental and physical stress, and medications, a repeat morning T concentration provides confirmatory evidence that the low T level is probably persistent. It should be noted that after oral testosterone undecanoate administration, the high levels of testosterone undecanoate in the blood can be cleaved by non-specific esterases ex vivo, so a blood collection tube with inhibitors of non-specific esterases (plasma) [34] should be used or more conveniently a conversion factor (serum T = plasma T/1.2) be applied to calculate serum T concentrations [35].



1652453610909.png





1.5 What Is Free Testosterone?

In men, T and estradiol circulate bound tightly to the sex hormone-binding globulin (SHBG) and loosely to albumin, and they also circulate in a free or unbound form. This led to the free hormone hypothesis postulating that free and the loosely bound testosterone or estradiol can freely diffuse out to the capillaries into the cells of the target tissues to initiate appropriate responses to these sex hormones [36]. SHBG is a glycoprotein synthesized in the liver with high-affinity binding sites for T and estradiol [37, 38]. In men, about 50–55% of testosterone is bound to SHBG, and the rest to albumin (45–48%), and the fraction of free testosterone is <2%. SHBG concentrations are affected by a number of factors (Table 1.3) [39]. Androgens (testosterone and its esters) and androgenic progestins (levonorgestrel, desogestrel, and progestins commonly used in female contraceptive pills) decrease SHBG levels. SHBG concentration is a good biomarker for androgen activity in the body. TD men have higher SHBG concentrations which decrease with androgen treatment. Since total T concentration is a measure of both bound and free testosterone, conditions, where SHBG may be increased or decreased, will affect the total T concentration. It is under these conditions that measurement of free T concentrations may be warranted (Table 1.3) [39]. For example, in an older overweight man with some symptoms of TD, aging increases and obesity decreases SHBG; in such circumstances, thus, to assess whether the older man has TD, measurement of serum-free T may be indicated. Free T measurements may also be helpful in symptomatic men with borderline low T concentrations, e.g., between 250 and 350 ng/dL (8.7–12.2 nmol/L) [7]. The binding of T to SHBG is complex, which results in many different methods that directly measure or calculate free T. Some of these methods do not measure the free fraction of T and some formulae may provide less accurate results [40].


Table 1.3 Factors that affect SHBG concentrations
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1.6 Are There Reliable Methods to Estimate Free Testosterone Concentrations?

The different methods of estimating free testosterone are shown in Table 1.4.


Table 1.4 Methods to measure serum-free testosterone
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1.6.1 Free Testosterone by Equilibrium Dialysis

Free T can be measured by equilibrium dialysis where test serum or plasma is mixed with isotope-labeled T and dialyzed overnight into a buffer solution. The free non-protein-bound fraction of the labeled T outside of the dialysis cell is the active “free fraction” of T. The free fraction (percent free T, usually between 1 to 2%) is multiplied by the total T measured by a reliable method to provide the free T concentration [41, 42]. This gold standard method of measuring free T by equilibrium dialysis is not automated, is cumbersome, and requires technical skill. Equilibrium dialysis methods are too complex for use in routine clinical chemistry laboratories. The methods are not harmonized and thus there are no common reference intervals to help clinicians to interpret free T concentrations [44]. Using this method, it has been found that concentrations of free T are normal even when the total testosterone is low in clinical conditions such as obesity [43] and other circumstances where SHBG is abnormal. Ultrafiltration methods are simpler but are sensitive to temperature changes, difficult to standardize with reproducible data, and, therefore, are not commonly utilized today [45]. Recent studies indicate that the method has better consistency in some laboratories, and their usefulness as a modified methodology will need further validation across laboratories [46, 47].




1.6.2 Bioavailable Testosterone

The concept of bioavailable T is based on the theory that the free fraction and the loosely albumin-bound fraction of circulating T are available to the target organs and tissues [48]. Thus, not only the free but also the albumin-bound T is biologically active in tissues. Bioavailable T – the sum of albumin-bound and free testosterone – is generally measured in the serum after adding saturated ammonium sulfate solution to precipitate the SHBG-bound fraction. The separation of SHBG-bound testosterone can also be done by adding concanavalin A [49]. These methods are not automated and standardized and thus not generally available in routine laboratories but are available in reference laboratories [44]. These methods require accurate and precise measurement of T in the non-SHBG bound fraction after ammonium sulfate precipitation or ultracentrifugation. Measurement of bioavailable T may be useful in men whose SHBG binding or concentration may be abnormal such as in older [50] and obese men [50].In most men with TD, measurement of bioavailable T is not usually required for diagnosis [51].




1.6.3 Salivary Testosterone

Because saliva does not contain SHBG, salivary T has been used as a surrogate for serum-free T [52, 53]. Salivary T can be measured by immunoassays or LC-MS/MS [54]. The concentration of T in the saliva may be influenced by the flow and also the presence of blood in the sample. For these reasons and non-familiarity with the use of saliva as a matrix, this simple method is not commonly used for free T determinations [55]; exceptions include the use of salivary T in studies on athletes and prepubertal children and infants where a blood draw can be avoided [56–58].




1.6.4 Calculated Free and Bioavailable Testosterone

Because of the technical difficulty, lack of automation, and absence of reference intervals for free T measured by equilibrium dialysis and bioavailable testosterone measured by ammonium sulfate precipitation methodologies (described above), these methods may not be suitable nor available in most routine clinical chemistry laboratories. This creates a widely utilized niche for calculated free T determinations. Calculated free and bioavailable T can be determined by using accurate and precise assays of T and SHBG [50, 59, 60]. Using different equations/algorithms, both free and bioavailable T may be calculated [59, 60], which have been recommended as suitable for routine clinical use [18, 44, 59]. The most commonly used equations based on the law of mass action [41, 60–62] are used to calculate both the free and bioavailable T. Other investigators have recommended the use of empirically derived equations that fitted the clinical populations studied [63, 64]; but these empirical equations are not widely used. The calculated free T using the law of mass action formula overestimates free T measured by equilibrium dialysis. Empirical formulae are free from assumptions and may be more concordant with the measured free T [63]. Recent evidence suggests that the law of mass action formula which is based on the assumption that two T molecules bind to two binding sites on the SHBG with similar binding affinity may be incorrect. And further argues that the binding of T to SHBG may be a multistep, dynamic process with complex allosteric characteristics [65]. Based on this new model, investigators used a new formula to calculate free T in younger men in the Framingham Heart Study and showed that the newly calculated values were similar to those measured by equilibrium dialysis. They further verified that the calculated free T values had clinical diagnostic validity using data from the European Male Aging Study. They demonstrated that men with calculated free T below the reference range had a higher risk of sexual symptoms and elevated LH suggestive of primary TD. While enticing, the use of this new formula must be further validated by other laboratories. The Endocrine Society suggests that calculated free T may be the most practical method to measure free T using accuracy and precise total T and SHBG measurements [7, 18]. Currently, the CDC is developing a harmonized method for free T based on calculated free T using revised formulae. This may bring the measurement of free T to a referable standard in clinical laboratories and common reference intervals that all clinicians can use.




1.6.5 Analog-Based Immunoassays and Why They Are Not Recommended by Most Experts in the Field

Analog-based free T assays are offered by most clinical laboratories, are measured on automated platforms, and are widely used by clinicians. However, many studies have shown that free T concentrations measured by analog-based immunoassay are about one-fifth of the concentrations measured by equilibrium dialysis and are related to SHBG [59, 66] or total T concentration [67], and do not reflect free T concentrations in clinical conditions such as hirsutism and hyperthyroidism [18, 68]. Experiments using varying concentrations of SHBG and T showed that analog-based free T immunoassays reported free T results that were related primarily to total T and concluded that free T analog assays do not detect serum-free T [67]. Some argue that free T concentrations measured by immunoassays are as good as calculated free T but failed to note that the free T values obtained by immunoassays are only 1/7 of those measured by equilibrium dialysis indicating clearly what is measured by the analog free T assays is not free T [69]. The Endocrine Society Position Statement indicates that analog-based assays have poor accuracy, sensitivity, and poor correlation with the equilibrium dialysis method [18]. Free T by analog immunoassay correlates with total serum T and provides no additional information and is not a measure of free T and should not be used.




1.7 Does Measurement of Free Testosterone Provide Additional Information for Clinical Diagnosis?

In most instances for the diagnosis of TD, total T measured in the morning should suffice if the concentrations are repeatedly below the reference range of the laboratory. In circumstances where the concentration of serum SHBG may be affected by liver or kidney disease, thyroid dysfunction, or other endocrine disorders (Table 1.3), the measurement of free T either calculated or by equilibrium dialysis may be warranted. For most clinicians, free T may be useful when older, overweight men with some symptoms suggestive of TD have serum T concentrations in the borderline range (e.g., between 250 and 350 ng/dL or 8.7 and 12.2 nmol/L). Aging is associated with a decrease in total serum T levels and an increase in SHBG, resulting in a greater decrease in free T, provided men are not obese. This is because obesity results in lower SHBG and lower total T, but the free testosterone concentration may be normal [43]. In a large population-based study (European Male Aging Study, 3349 men aged 40–79 years), men with normal total but low calculated free T were older with poorer health and exhibited more sexual symptoms, whereas those with low total T and normal free T were more obese and had no features of androgen deficiency. The results suggested that older men with lower free T have symptoms suggestive of androgen deficiency, despite having normal total T levels [70]. Furthermore compared to older obese men with low total T and normal or low luteinizing hormone (LH), men who have low free T had more sexual symptoms including lower sexual desire and infrequent morning erections, which suggests that low free T may be indicative of symptomatic TD [71]. The Testosterone Trials in which older men with symptomatic TD were administered placebo or T gel daily for a year showed that baseline total and free T were significantly and independently associated with sexual desire, erectile function, and sexual activity but not with vitality or physical function [72]. In addition, after treatment with T gel, the improvements in sexual activity and desire were associated with both serum total T and free TD, indicating that the sexual function improvement was related to the incremental increases of both serum total T and free T [73]. These studies indicate that in older men with symptoms suggestive of TD, measurement of free T may be indicated even when total T concentration may be normal. Perhaps the newer formula for calculated free T validated in multiple laboratories [65], will become generally available, correlate with free T by equilibrium dialysis and demonstrate improved correlation with clinical symptoms and therapeutic responsiveness. If all these prove to be true, then this formula to calculate free T may be a justified replacement for free T measurement by the equilibrium dialysis methodology.




1652456777539.png
 
Defy Medical TRT clinic doctor
*The binding of T to SHBG is complex, which results in many different methods that directly measure or calculate free T. Some of these methods do not measure the free fraction of T and some formulae may provide less accurate results [40]

*
Recent evidence suggests that the law of mass action formula which is based on the assumption that two T molecules bind to two binding sites on the SHBG with similar binding affinity may be incorrect. And further argues that the binding of T to SHBG may be a multistep, dynamic process with complex allosteric characteristics [65]. Based on this new model, investigators used a new formula to calculate free T in younger men in the Framingham Heart Study and showed that the newly calculated values were similar to those measured by equilibrium dialysis. They further verified that the calculated free T values had clinical diagnostic validity using data from the European Male Aging Study

*Currently, the CDC is developing a harmonized method for free T based on calculated free T using revised formulae. This may bring the measurement of free T to a referable standard in clinical laboratories and common reference intervals that all clinicians can use


*Perhaps the newer formula for calculated free T validated in multiple laboratories [65], will become generally available, correlate with free T by equilibrium dialysis and demonstrate improved correlation with clinical symptoms and therapeutic responsiveness. If all these prove to be true, then this formula to calculate free T may be a justified replacement for free T measurement by the equilibrium dialysis methodology




Phase II: Research and Commercialization of TruT Algorithm for Free Testosterone

Jasuja, Ravi



The measurement of testosterone (T) levels is central to the diagnosis of androgen disorders, such as hypogonadism in men and polycystic ovary syndrome (PCOS) in women. Circulating T is bound with high affinity to sex hormone-binding globulin (SHBG) and with substantially lower affinity to albumin; only the free fraction is biologically active. Conditions that affect SHBG concentrations, such as aging and obesity, alter total but not free T concentrations; in these conditions, the determination of free T is necessary to obtain an accurate assessment of androgen status. The tracer analog method, the most widely used method for free T, has been shown to be inaccurate. The equilibrium dialysis method, considered the reference method, is technically difficult to implement and standardize, and is not available in most hospital laboratories, leading the Endocrine Society's Expert Panel to conclude that ?? the calculation of free testosterone is the most useful estimate of free testosterone in plasma?? Therefore, there is an unmet need for algorithms that provide accurate estimates of free T that match those derived from equilibrium dialysis. We have designed a novel and accurate TruTTM algorithm for the determination of free T, based on the characterization of testosterone's binding to SHBG using modern biophysical techniques. We have discovered that testosterone's binding to SHBG is a dynamic multistep process that includes allosteric interaction between the two binding sites on an SHBG dimer. Our computational framework incorporates the correct binding parameters derived experimentally in these studies, the non-linear dynamics in T: SHBG association, and allostery

In phase I studies, we demonstrated that the TruTTM algorithm provides accurate free T values that match those obtained using the equilibrium dialysis in healthy and hypogonadal men
. We have also shown that the binding parameters that have formed the basis of previous equations (e.g., Vermeulen) are incorrect, and that free T values derived using these equations deviate substantially from free T measured by equilibrium dialysis. The phase I studies have led to the adoption of the TruTTM algorithm at several institutions.

The phase II program will continue the development of the TruTTM algorithm by validating it in common conditions characterized by altered SHBG concentrations, such as obesity and aging (AIM 1), in healthy women across the menstrual cycle, and in women with PCOS (Aim 2).
We will generate population-based reference ranges for free T (Aim 3). Phase II also includes plans for the commercialization of the TruTTM algorithm using a HIPAA-compliant infrastructure for its clinical adoption

The phase II program will provide validation of the TruTTM algorithm in the two most common clinical indications for free T measurement? men suspected of hypogonadism and altered SHBG levels, and women with hyperandrogenic disorders. It will also enable the development of a HIPAA-compliant platform that can be embedded into the electronic medical record for wider clinical adoption and for improving clinical care
 
*Currently, the CDC is developing a harmonized method for free T based on calculated free T using revised formulae. This may bring the measurement of free T to a referable standard in clinical laboratories and common reference intervals that all clinicians can use
 
"" Equilibrium dialysis methods are too complex for use in routine clinical chemistry laboratories.""

Are they saying that we (everyday lab consumer) shouldn't be trying to get our free T measured by equilibrium dialysis at this point? FWIW: I'm with Defy. They still use the standard lab for determining free T

How do you all feel about the TruT Free Testosterone Calculator by FPT online calculator? Is it good enough for most cases?
 
"" Equilibrium dialysis methods are too complex for use in routine clinical chemistry laboratories.""

Are they saying that we (everyday lab consumer) shouldn't be trying to get our free T measured by equilibrium dialysis at this point? FWIW: I'm with Defy. They still use the standard lab for determining free T

How do you all feel about the TruT Free Testosterone Calculator by FPT online calculator? Is it good enough for most cases?

My 2 cents...

 
"" Equilibrium dialysis methods are too complex for use in routine clinical chemistry laboratories.""

Are they saying that we (everyday lab consumer) shouldn't be trying to get our free T measured by equilibrium dialysis at this point? FWIW: I'm with Defy. They still use the standard lab for determining free T

How do you all feel about the TruT Free Testosterone Calculator by FPT online calculator? Is it good enough for most cases?

No.

You should still be using what would be considered the most accurate assays for testing free testosterone such as the gold standard Equilibrium Dialysis or Ultrafiltration (next best), especially in cases of altered SHBG.

Use the same lab (reliable) and same assay (most accurate) every time you have blood work done.

For the time being until the limitations of testing free testosterone by (ED/UF) are addressed, you will have to put faith in the lab you are using.


* Limitations of using free testosterone by equilibrium dialysis and calculated free testosterone concentrations in practice are the lack of assay standardization, an accuracy-based quality control program, and a harmonized reference range. Until these limitations are addressed, free testosterone by equilibrium dialysis and calculated free testosterone should use reference ranges established by individual laboratories or their specific assay method

*Assays that are standardized are designed to provide accurate results, traceable to “true” value-assigned certified reference materials and gold-standard reference methods. Results obtained using standardized methods can be compared across assays, institutions, populations, and past and future test results, thereby improving diagnosis, treatment, and outcomes of patients




post #4


28:50-32:38

(29:20-30:05)
We are working with different organizations on developing reference intervals that are based on certified assays. So we did already that successfully for testosterone.

We are currently working with some groups (research groups) on free testosterone reference intervals.

Screenshot (13088).png






*Measuring FT is technically challenging and shows high variability. The CDC clinical standardization program is developing a high throughput method using the gold-standard equilibrium dialysis (ED) procedure with isotope dilution ultra-high-performance liquid chromatography-tandem mass spectrometry (ID-UHPLC-MS/MS).




post #38

CDC Hormone Standardization Program (CDC HoSt) Certified Free Testosterone Procedures?

Sooner or later and SHBG to boot!

When the time comes these will be the only free testosterone assays I will recommend for men to use/rely upon when getting blood work done (pre/post-TRT).


*a lab/assay that is certified by the CDC's HoSt Program
Screenshot (13089).png


The above applies to TT, estradiol, and soon enough free testosterone and SHBG!



*Assays that are standardized are designed to provide accurate results, traceable to “true” value-assigned certified reference materials and gold-standard reference methods. Results obtained using standardized methods can be compared across assays, institutions, populations, and past and future test results, thereby improving diagnosis, treatment, and outcomes of patients

* Limitations of using free testosterone by equilibrium dialysis and calculated free testosterone concentrations in practice are the lack of assay standardization, an accuracy-based quality control program, and a harmonized reference range. Until these limitations are addressed, free testosterone by equilibrium dialysis and calculated free testosterone should use reference ranges established by individual laboratories or their specific assay method




post #8


*Free testosterone concentration is ideally measured using the equilibrium dialysis method, performed under standardized conditions.1,31

*Direct tracer analog methods for measuring free testosterone concentrations are inaccurate, and therefore, their use is not recommended.35


*equations that are based on a linear model of testosterone’s binding to SHBG assume a fixed binding affinity (approximately 1 nM)31 and ignore the competing presence of other sex steroids, such as dihydrotestosterone and estradiol

*Recent studies using modern biophysical techniques have suggested that the binding of testosterone and estradiol to an SHBG dimer is a dynamic process that involves allosteric interactions between binding sites on each of the 2 SHBG monomers such that the binding affinities of the 2 sites are not equivalent.36,39 The binding of a ligand to the first monomer influences the conformational and energetic states of both the monomers.39 The estimation of free testosterone concentration based on an ensemble allosteric model provides a close approximation of concentrations measured using equilibrium dialysis36;

*the computations of free testosterone concentrations using the ensemble allostery model can be obtained at TruT Free Testosterone Calculator by FPT

*Because of dynamic changes in the binding affinity of SHBG upon ligand binding, depending on the ligand and SHBG concentrations, no equation can accurately estimate free testosterone concentration under all conditions.39






24:05-37:00 (video)

28:36-31:58 (cFTV/cFTZ)

Shalender Bhasin :

*the calculated free testosterone is based on the simplistic notion that total testosterone is linearly related to free testosterone concentration and so you can compute total testosterone if you know the binding affinity and the concentrations of SHBG and albumin discounting orosomucoid and cortisol binding globulin and many people just ignore albumin because of the perception that albumin-bound testosterone remains relatively in constant

*and there are some empirically derived equations

*and I'll show you that the linear equations such as the Vermeulens equation that is based on the simplistic idea that one molecule of testosterone binds to one molecule of SHBG at a single binding site with a fixed binding affinity of 1 nanomolar (nM) to form a testosterone SHBG complex

*what are studies have shown is that testosterone binding to SHBG and we have shown similar data with estradiol which I'll show you in a minute

*and that this binding is a multi-step dynamic process

*so SHBG circulates as a dimer in circulation and this dimer is very tightly bound and it takes 8 nanomolar (nM) to dissociate the dimer but upon binding of the first testosterone to the first binding pocket in the first monomer there's a change in conformation of the first monomer as well as change in the conformation of the second monomer due to the allosteric interaction between the two binding pockets such that the binding of testosterone to the second binding pocket in the second monomer occurs with a different binding affinity and this process is very dynamic so the Kd is not fixed therefore the linear equations such as the Vermeulen equation and others that assume a fixed Kd are just conceptually wrong and our data show it clearly that this model is completely wrong

*so the Vermeulen model or most of the linear equations underestimate free testosterone concentrations and the ensemble allosteric model (EAM) based upon our experimental data matches total testosterone within the range in which we have validated this

*so let me show you some additional data which persuade me that no equation can ever be an accurate measure of the free testosterone at all levels of SHBG, testosterone, estradiol, DHT, and albumin under all conditions in men in women





My reply from an earlier thread:

post #16

The EAM appears to be an accurate and testable model for calculating free testosterone levels, but this model needs further validation in large populations.

This will be a part of the ongoing phase II.




post #14


As I have stated numerous times on the forum!

Patiently waiting on the completion of Phase II for the TruT (cFTZ) Algorithm let alone standardization and harmonized reference ranges for Free testosterone which is in the works as we speak.

Phase II should be coming to an end soon enough.

8 years in 2014-2022.

Ravi let alone Shalender is confident about the validity/soon-to-be commercialization of the TruT Algorithm.

It's going to happen.

He is already pushing the use of the newer calculated method! (Testosterone Deficiency in Men)

Much going on behind the scenes and more to come.








One of Bhasin's current papers.


*Free testosterone concentration is ideally measured using the equilibrium dialysis method, performed under standardized conditions.1,31 Direct tracer analog methods for measuring free testosterone concentrations are inaccurate, and therefore, their use is not recommended.35 Although several equations to estimate free testosterone concentration from total testosterone, SHBG, and albumin concentrations have been published,36-38 the estimation of free testosterone concentration performed using these equations are predicated upon accurate measurements of total testosterone, SHBG, and albumin concentrations.31,35 Furthermore, equations that are based on a linear model of testosterone’s binding to SHBG assume a fixed binding affinity (approximately 1 nM)31 and ignore the competing presence of other sex steroids, such as dihydrotestosterone and estradiol.

*Recent studies using modern biophysical techniques have suggested that the binding of testosterone and estradiol to an SHBG dimer is a dynamic process that involves allosteric interactions between binding sites on each of the 2 SHBG monomers such that the binding affinities of the 2 sites are not equivalent.36,39 The binding of a ligand to the first monomer influences the conformational and energetic states of both the monomers.39 The estimation of free testosterone concentration based on an ensemble allosteric model provides a close approximation of concentrations measured using equilibrium dialysis36;

*the computations of free testosterone concentrations using the ensemble allostery model can be obtained at TruT Free Testosterone Calculator by FPT. Because of dynamic changes in the binding affinity of SHBG upon ligand binding, depending on the ligand and SHBG concentrations, no equation can accurately estimate free testosterone concentration under all conditions.39




Phase II: Research and Commercialization of TruT Algorithm (Sep.15, 2014-May 31, 2022)
Screenshot (13090).png





They have most likely wrapped up Phase II and it is just a matter of time before the data comes out.

For the time being, do what you feel is best for you.

Just make sure to steer clear of using/relying upon the piss poor direct immunoassay!
 
Hi I'm in Canada and just had my blood taken from Dynalab. When I asked what method they used to test TT, FT and Estradiol sensitive they could not give me an answer.
1. Does anyone know where I can find out? Their website wasn't helpful.
2. If all my results are from the same lab can I assume that the following results are relative? For example, can I use the first years results as a reference for any following labs? So I may not know if the numbers are accurate I will know if my levels have risen, fallen, or stayed the same?
 
They have most likely wrapped up Phase II and it is just a matter of time before the data comes out.

For the time being, do what you feel is best for you.

Just make sure to steer clear of using/relying upon the piss poor direct immunoassay!
Thanks for chiming in Madman. I will be making an effort to remind DEFY use the EQ dialysis method next time they book my labs. They're still having everyone do direct immunoassay. I am assuming that Labcorp has EQ dialysis.
 
Thanks for chiming in Madman. I will be making an effort to remind DEFY use the EQ dialysis method next time they book my labs. They're still having everyone do direct immunoassay. I am assuming that Labcorp has EQ dialysis.
Until CDC shows fT methods have been Harmonized I still don't get using ED method.

I will stick to cfTV*0.8 to get within spitting distance of what ED puts out. You can also bracket with cfTV and cfTZ and do the direct RIA fT transform. Compare all three against your Labcorp ED result for fun. And then save all that subsequent money on ED measurements until there are certified ED labs.




Post in thread 'Calculate free testosterone with TruT by FPT' Calculate free testosterone with TruT by FPT
 
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