Biochemical examination in hyperlipoproteinemia

In recent years, the issue of lipid metabolism disorders has come to the forefront of interest, especially in connection with the prevention and treatment of cardiovascular diseases. Biochemical examinations play an important role in the diagnosis of hyperlipoproteinemias and the monitoring of therapy.

The basic laboratory examination  is the determination of total cholesterol and triacylglycerols in serum (plasma), as well as the determination of LDL- and HDL-cholesterol.

Other more specialized examinationsinclude the determination of typical apoproteins apoA-I (HDL) and apoB-100 (LDL),or lipoprotein (a) and depleted lipoproteins electrophoresis. DNA diagnostics is also gradually developing, affecting the causes of some HLP.

Laboratory diagnosis of lipid metabolism disorders must be based on examination of blood lipids from at least two blood samples in the range of 2-8 weeks, under normal lifestyle. Differences are found for each parameter and, if lower than the allowable values, an arithmetic mean is calculated for each analyte. If the critical difference between 2 consecutive analyzes is exceeded, a third examination is performed.


 * {| class = wikitable


 * + Critical differences for lipid metabolism analytes

! Analyte !! Critical difference [%]
 * align = center | Total cholesterol || align = center | > 20
 * align = center |LDL-cholesterol||align = center | > 25
 * align = center |HDL-cholesterol ||align = center | > 25
 * align = center |Triacylglycerols||align = center |> 65
 * }
 * align = center |HDL-cholesterol ||align = center | > 25
 * align = center |Triacylglycerols||align = center |> 65
 * }
 * }

It should also be taken into account that the examination of lipid metabolism is significantly affected by lifestyle (dietary habits, physical activity, body weight), pharmacotherapy (hormonal contraception, hormone replacement therapy, etc.) and ongoing acute or uncompensated disease. Therefore, blood lipid testing should not be performed when it can be assumed that the result will not indicate a situation in a normal lifestyle (shortly after vacation, during hospitalization for other reasons, acute diabetes mellitus, during pregnancy and half a year after, etc.).

Principle
270px|thumb|Obr. 2 Stanovení celkového cholesterolu Cholesterol is transported in blood plasma as part of lipoproteins, mostly in the LDL fraction, less so in HDL and VLDL. Of this cholesterol, approximately two-thirds is esterified with higher fatty acids, the remainder being unesterified.
 * Serum (plasma) is routinely determined for total cholesterol.Therefore, the actual determination of total cholesterol is preceded by the hydrolysis of cholesterol esters to free cholesterol and fatty acids by the enzym cholesterolesterase (CE).
 * NThis is followed by oxidation of non-esterified cholesterol to 4-cholesten-3-one to form hydrogen peroxide in a cholesterol oxidase (CHOD)catalyzed reaction.
 * The later reaction uses hydrogen peroxide to oxidatively couple 4-aminoantipyrine and phenol in the presence of another enzyme peroxidase (POD).A colored product is formed whose absorbance is proportional to the amount of cholesterol (Fig. 2).

Evaluation

 * The risk of atherosclerosis increases  with increasing total cholesterol levels. According to Czech and European recommendations, the concentration of total cholesterol should be <5.0 mmol / l. Total cholesterol should be determined in all people over the age of 18 as part of prevention. The test should be repeated in 5 years even in the case of a normal result, i.e. up to 5.0 mmol / l.


 * If the concentration is higher and also in patients with ischemic heart disease and other high-risk individuals, we proceed to a more detailed examination of the lipid spectrum by determining LDL- and HDL cholesterol and triacylglycerols.


 * In patients at increased risk of cardiovascular disease (eg diabetics), total cholesterol should be lower <4.5 mmol / l and in people with already manifest cardiovascular disease even <4.0 mmol / l.


 * Elevated cholesterol levels are also often found in diabetics or hypothyroidism. Total cholesterol levels are reduced, for example, in advanced liver cirrhosis or hyperthyroidism or malnutrition.


 * It is a marker for overall mortality and a risk factor for CVD. The relationship of cholesterol to overall mortality is non-linear, J-shaped or U-shaped, which can be explained by the mechanism of reverse causality.

Evaluation limits
Serum total cholesterol (total S-cholesterol): 2,9–5,0 mmol/l.

Principle
LDL-cholesterol levels can be determined indirectly by calculation or directly by analysis.

Indirect determination of LDL-C

 * The so-called Friedewald's formula is used for the indirect determination of LDL-C.
 * LDL-cholesterol = total cholesterol – HDL-cholesterol – TG/2,2


 * It is based on the assumption that serum cholesterol is contained in the HDL, LDL and VLDL fractions. The calculation requires the measurement of three different analytes - total cholesterol, HDL-cholesterol and triacylglycerols. This increases the possibility of analytical errors. We determine total cholesterol and HDL-cholesterol directly. Cholesterol detection in VLDL is difficult. We determine it on the assumption that the molar ratio of cholesterol in VLDL is on average 45% of the total triacylglycerol content; then the TG / 2.2 fraction represents cholesterol in the VLDL particles. The formula can only be used if the value of triacylglycerols does not exceed 4.5 mmol / l, chylomicros must not be present.

Direct determination of LDL-C
Direct determination of LDL-cholesterol by homogeneous methods is gradually being introduced into practice without the need for separation steps and centrifugation, the advantage of which is the possibility of automation. Simplification of the analysis has been achieved by the use of various detergents and other reagents that specifically block or dissolve individual lipoprotein fractions. In this way, the LDL particles are separated and the cholesterol content is determined in the final phase of the analysis. 270px|thumb|Obr. 3A Přímé stanovení LDL-cholesterolu 270px|thumb|Obr. 3B Přímé stanovení LDL-cholesterolu

Several procedures have been developed for the direct determination of LDL-C. The analysis is usually divided into two steps.


 * One method uses various detergents and other substances to selectively block cholesterol in non-LDL particles (HDL, VLDL and chylomicrons), whose cholesterol becomes inaccessible to the enzymes used to determine it. Cholesterol is determined in unblocked LDL particles after release by the enzyme method described for total cholesterol using the cholesterolesterase, cholesterol oxidase and peroxidase reactions (Fig. 3A).

There are also other methods for determining direct LDL-cholesterol.
 * In another method, cholesterol is released from chylomicrons, VLDL and HDL in a first phase using a detergent. The released cholesterol is converted by enzymes to 4-cholesten-3-one and hydrogen peroxide. The hydrogen peroxide formed at this stage is not used to form a colored product, as it would interfere in the next step of the determination. Therefore, it is decomposed by catalase into water and oxygen. In this reaction, no color develops. In the second phase, another detergent releases cholesterol from the LDL, which is then determined similarly to total cholesterol (Fig. 3B).

Evaluation

 * Elevated LDL-cholesterol levels significantly contribute to the development of atherosclerosis. According to current Czech and European recommendations, the recommended concentration of LDL-cholesterol is < 3,0 mmol/l.
 * LDL concentrations <2.6 mmol / l are recommended for patients at increased risk of cardiovascular disease and <1.8 mmol / l for patients with already developed cardiovascular disease.

Evaluation limits
Serum LDL-cholesterol: 1,2–3,0 mmol/l

Principle
Older methods for HDL-C determination

Older methods use procedures based on the determination of cholesterol in HDL particles after removal of non-HDL particles. The precipitated lipoprotein particles are separated by centrifugation. The cholesterol concentration in the HDL particles in the supernatant is then determined using commonly used photometric methods.

Direct determination of HDL-C
Modern, easily automated methods use, as with LDL-C, the direct determination of HDL-cholesterol using homogeneous methods without precipitation and centrifugation. Several procedures have been developed for the direct determination of HDL-C. The analysis is usually divided into two steps.

270px|thumb|Obr.4A Přímé stanovení HDL-cholesterolu imunoinhibicí 270px|thumb|Obr.4B Přímé stanovení HDL-cholesterolu


 * In the first step, all non-HDL particles (VLDL, LDL, chylomicrons) are blocked. By blocking the non-HDL particles, the reaction of the cholesterol contained in them with the enzymes used for its determination is prevented. Blockade can be achieved by immunoinhibition with antibodies directed against apoB, which is part of VLDL, LDL and chylomicrons. Antibodies form soluble immunocomplexes with non-HDL. In the next step, the detergent dissolves the HDL particles and the cholesterol in the HDL is measured by the enzymes cholesterol esterase, cholesterol oxidase and peroxidase in the same way as in the determination of total cholesterol, i.e. by the enzymes (Fig. 4A).


 * Another method is used to block polyanions and polymers that selectively adsorb to the surface of non-HDL lipoproteins. These are then protected against detergents which release cholesterol contained only in HDL particles. The second step of the analysis is analogous to the procedure described in the first method (Fig. 4B).

Evaluation

 * HDL-cholesterol levels should be > 1,0 mmol/l in men and > 1,2 mmol/l in women. Elevated HDL-C is considered a „negative risk“ factor for the development of atherosclerosis, and conversely, levels below 1.0 mmol / l are associated with an increased risk of atherosclerosis.
 * Low HDL is accompanied by metabolic syndrome, low physical activity, type 2 DM, cigarette smoking and consumption of large amounts of carbohydrates.

Evaluation limits

 * Serum HDL-cholesterol (males): 1,0–2,1 mmol/l


 * Serum HDL-cholesterol (females): 1,2–2,7 mmol/l

Determination of triacylglycerols
270px|thumb|Obr.5 Stanovení triacylglycerolů

Principle
Recommended routine methods for the determination of triacylglycerols use several enzymatic reactions.


 * Lipoprotein lipase catalyzes the hydrolysis of triacylglycerols to glycerol and fatty acids.
 * The released glycerol is converted by glycerol kinase in the presence of ATP to glycerol-3-phosphate, which is oxidized to dihydroxyacetone phosphate by glycerol-3-phosphate oxidase.
 * The co-formed hydrogen peroxide is used in anotherperoxidase-catalyzed reaction to oxidatively couple 4-aminoantipyrine with a phenol derivative. A quinone imine dye is formed, the absorbance of which is deducted.

Evaluation

 * Elevated triacylglycerol levels are an independent risk factor for atherosclerosis. ČCzech and European recommendations consider a normal serum triacylglycerol concentration to be < 1,7 mmol/l.
 * TG concentration> 1.7 mmol / l (fasting) is considered an indicator of increased cardiovascular risk. Higher triacylglycerols are associated with decreased HDL levels and predict high concentrations of cholesterol-rich remnants and small dense B-type LDL particles.
 * The concentration of triacylglycerols increases within 2 hours after a meal and reaches a maximum in 4-6 hours, therefore blood must be collected for the determination of triacylglycerols after 12-14 hours of fasting. Plasma samples with a TG concentration higher than 3.4 mmol / l opalesce, chylomicrons are present at TG levels above 11.3 mmol / l and the plasma is milky turbid.
 * Therapy places great emphasis on a diet low in fat and sugar, increased physical activity, plenty of antioxidants in the diet and overall hypolipidemic treatment.

Evaluation limits
Serum triacylglycerol concentration (fS-triacylglycerols): 0,45–1,7 mmol/l

Odvozené parametry lipidového metabolismu
Cílem těchto výpočtů je zpřesnit stanovení rizika, které vyplývá z naměřených hodnot krevních lipidů.

Aterogenní index

 * Z naměřených hodnot týkajících se cholesterolu lze počítat různé aterogenní indexy. Doručován je index, který bere v úvahu vliv koncentrace celkového cholesterolu i HDL-C na riziko kardiovaskulárních onemocnění. Index zohledňuje fakt, že zvýšený HDL-C je „negativní rizikový faktor“, snižující riziko ischemické choroby srdeční (ICHS). Současné zvýšení celkového i HDL cholesterolu nemusí riziko ICHS zvyšovat.


 * Celkový cholesterol/HDL-cholesterol

Doporučená hodnota
Aterogenní index: < 5,0

Non-HDL-cholesterol

 * Je využíván k odhadu rizika aterosklerózy v případech, kdy není možno vypočítat koncentraci LDL-C. Představuje cholesterol obsažený v potenciálně aterogenních lipoproteinových částicích (LDL, IDL, VLDL, zbytkové chylomikrony).
 * Non-HDL-cholesterol (mmol/l) = celkový cholesterol (mmol/l) – HDL-cholesterol (mmol/l)

Doporučená hodnota
Non-HDL-cholesterol: < 3,8 mmol/l

Chylomikronový test
Princip: thumb|250px|Obr. 6 Vzhled séra při chylomikronovém testu
 * Měření koncentrace chylomikronů není běžně prováděno. Ve vzorcích odebraných po 12 hodinovém lačnění by se neměly vyskytovat. Pro jejich přítomnost svědčí silná chylozita séra. K důkazu lze provést chylomikronový test, který spočívá v pozorování opalescentního až bílého prstence po 12ti hodinovém stání séra při 4 °C. Během této doby flotují eventuálně přítomné chylomikrony k hladině vzorku. Každé zdravé sérum má být po 12 hodinovém lačnění úplně čiré.
 * Vzhled séra při chylomikronovém testu může upozornit i na jiné poruchy v metabolismu lipoproteinů.

Princip

 * Lipoproteinové částice se dělí v elektrickém poli podle rozdílné velikosti povrchového náboje, v tomto případě podmíněného rozdílným množstvím bílkovin v jednotlivých frakcích. Využívá se především pro průkaz některých abnormálních lipoproteinů a při diagnostice méně častých typů hyperlipoproteinémií a pro detekci aterogenního lipoproteinu Lp (a).
 * Nejrychleji v oblasti &alpha; se pohybují nejmenší částice s nejvyšším obsahem proteinů &alpha;-lipoproteiny (HDL). Na úrovni mezi &alpha;-2 a &beta; jako pre-&beta;-lipoproteiny migrují VLDL částice. LDL částice představují obvykle nejvýraznější frakci jako &beta;-lipoproteiny v oblasti &beta;-globulinů. Chylomikrony, pokud jsou přítomny v séru, zůstávají na startu, někdy mohou vytvářet pruh, který je viditelný od místa startu až k &alpha; oblasti. V poloze mezi &alpha; a &beta;-lipoproteiny (HDL a LDL) se může objevit další frakce charakteristická pro lipoprotein (a) – Lp(a), který představuje rizikový faktor pro vznik aterosklerózy a kardiovaskulárních onemocnění.
 * Provedení elektroforézy sérových lipoproteinů je obdobné jako u elektroforézy sérových bílkovin s tím rozdílem, že k barvení se používají lipofilní barviva např. Sudanová čerň. Elektroforéza lipoproteinů se obvykle provádí na agarosovém gelu, který umožňuje dobré oddělení pre-&beta;-lipoproteinů.

Hodnocení

 * Elektroforeogram lze vyhodnotit denzitometricky při vlnové délce 580 nm. Výsledek se vyjadřuje v procentech optické hustoty pro jednotlivé frakce vzhledem k celkové barevné ploše. Stanovené hodnoty spolu s dalšími ukazateli (celkový cholesterol, triacylglyceroly) slouží k charakterizaci hyperlipoproteinémií (Obr. 7, 8, 9).


 * V praxi se provádí také hodnocení pouze vizuální. Biologický nález se srovnává s referenčními hodnotami a výsledek se posuzuje ve smyslu zvýšení (snížení) jednotlivých frakcí.

Související články

 * Dyslipidémie
 * Lipoproteiny (klinika)
 * Lipoproteiny
 * Hypolipidemika
 * Hypolipidemická léčba

Externí odkazy

 * Lipoproteiny (česká wikipedie)
 * Lipoprotein (anglická wikipedie)