OA20804A - A solution for measurement of Trehalase in urine and measurement method using this solution - Google Patents

A solution for measurement of Trehalase in urine and measurement method using this solution Download PDF

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OA20804A
OA20804A OA1202100539 OA20804A OA 20804 A OA20804 A OA 20804A OA 1202100539 OA1202100539 OA 1202100539 OA 20804 A OA20804 A OA 20804A
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urine
measurement
glucose
trehalase
solution
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OA1202100539
Inventor
Bidi Bülent
Olgun Abdullah
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Argeron Medi̇kal Araştirma Sanayi Ve Ticaret Anonim Şirketi
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Publication of OA20804A publication Critical patent/OA20804A/en

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Abstract

Invention relates to a trehalose solution for use with urinary glucose measurement kits, in in vitro diagnostic (biochemical medical diagnosis) field, to measure urinary trehalase enzyme activity as a marker of kidney damage, and a measurement method where the solution is used.

Description

DESCRIPTION
A solution for measurement of Trehalase in urine and Measurement method using this Solution
The Field ofthe Invention
Invention relates to a trehalose solution for use with urinary glucose measurement kits in in vitro diagnostic (biochemical medical diagnosis) field to measure urinary trehalase enzyme activity as indication of kidney damage, and a measurement method where this solution is used.
Background of the Invention
Trehalase is a glycoprotein structured enzyme of 75 kDa molecular weight and présent in rénal proximal tabules and intestines. Urinary trehalase measurement can be used for screening, diagnosis and monitoring of damage occurred in rénal proximal tubules It 15 is reported that trehalase activity was higher than the control group even when proteinuria and glucosuria are négative from the early stages of diabètes; and in late stages of diabètes, activity decreases because of disappearance of brush bordera in proximal tubules (3). It can show early kidney damage due to some environmental toxins. It was shown that trehalase activity was increased in comparison to control group in workers who 20 melt lead; there was a positive linear relationship between blood lead level and urinary trehalase activity. And in case of environmental cadmium exposure, a similar increase in activity was seen (4-6). It was reported that the use of ampicillin and tobramycin antibiotics in infants increased urinary trehalase activity (7). In chronic glomerular disease and particularly nephrotic syndrome, urinary trehalase activity increase was observed (8).
At présent there are various methods used for measurement of trehalase in urine. These methods are divided into two main groups, namely, those measuring trehalase enzyme activity (colorimétrie) and mass measuring ones (immunochemicai). However, there is no example developed as a kit commonly used in routine diagnostic laboratories. For that 30 reason, methods are needed particularly to provide early, fast, widespread and economical diagnosis of kidney damage .
As a resuit, due to above described disadvantages and inadequacy of existing solutions it has been necessary to make development in the related art,
Brief Description of the Invention
The present invention relates to urinary trehalase measurement meeting the needs mentioned above, eliminating ail disadvantages and providing some additional advantages.
Primary purpose of invention is to provide the use of kits already used for measurement of urinary glucose for urinary trehalase activity measurement also and thus allow very fast and widely satisfaction of need for trehalase measurement. Because contrary to urinary trehalase measurement, urinary glucose measurement is a routine measurement made in almost ail medical diagnostic laboratories ail around the world. The invention will enable the use of widely used urinary glucose measurements for urinary trehalase activity measurement also. There is no other product used for this purpose.
In order to achieve above mentioned purposes, the invention is a trehalose solution for use together with urinary glucose measurement kits for the measurement of urinary trehalase enzyme activity in biochemical diagnostic field. In a preferred application of the invention, said solution contains trehalose in a concentration range of 0,2 - 68,0 g/dL, preferably 40 g/dL. The invention also comprises urinary trehalase measurement kits containing said solution.
In order to achieve above mentioned purposes, the invention is a urinary trehalase enzyme measurement method wherein said solution is used and comprises following process steps:
a) Mixing trehalose solution and urine sample,
b) Incubating mixture at a predetermined température and duration,
c) Measurement of glucose in the mixture by glucose measurement kit using the selected urine,
d) Measurement of glucose in de-ionized water added urine mixture at said équivalent conditions in previous steps,
e) Evaluation of différence between two glucose measurement results.
According to an application of the invention, said trehalose solution in process step “a” contains trehalose in a concentration range of 0,2 - 68,9 g/dL, preferably 40 g/dL.
According to an application of the invention, in process step “a” 1 unit volume of trehalose 5 solution is mixed with 39 unit volume of urine.
According to an application of the invention, in process step “d 1 unit volume of deionized water is mixed with 39 unit volume of urine.
According to an application of the invention, in process step “e’’, trehalose solution and deîonized water are mixed and the différence between these two different urinary glucose 10 measurements is calculated as trehalase activity.
According to an application of the invention, in process step e, from the concentration of glucose formed by Trehalase enzyme, trehalase activity resuit is calculated as U/L.
According to an application of invention, in process step “e”, Trehalase activity producing 2 pmol glucose from 1 pmol trehalose per minute is assumed as Unit (U).
The structural and characteristic features of the invention and ail advantages will be understood better in detailed descriptions given below and therefore, the assessment should be made taking into account the figures and detailed explanations.
Detailed Description of the Invention
In this detailed description, the invention and preferred applications of the invention hâve 20 been described for the purpose of better understanding of the matter and in a manner not forming any restrictive effect.
The invention is a trehalose solution for use together with urinary glucose measurement kits for measurement of urinary trehalase enzyme activityin biochemical diagnostic field.
Trehalose solution of the invention provides use of kits used for urinary glucose measurement routînely ai medical diagnostic laboratories worldwide for urinary trehalase activity measurement too.
Trehalose contained in solution of the invention is added to urine. It is transformed into glucose by trehalase enzyme in urine.
The kit used for measurement of glucose in urine routinely can also measure glucose in urine having been added solution of the invention or deionized water. The différence between two different measurements with solution and deionized water added shows 5 trehalase activîty.
Urinary glucose measurement kits used under the invention also contains urinary analysis reactive dipsticks. It measures glucose formed in urine treated with trehaiose solution of the invention. Any type of commercial kits used routinely at medical diagnostic 10 laboratories can be used for measurement of glucose in urine by solution of the invention.
Method for measurement of trehalase enzyme in urine performed by solution of the invention comprises following processes steps in the most basic form.
- Mixing trehaiose solution and urine sample,
Incubatîng mixture at predetermined température and duration,
Measurement of glucose in mixture by glucose measurement kit with selected urine,
Measurement of glucose in de-ionized water added urine mixture at said 20 équivalent conditions in previous steps,
Evaluation of différence glucose results between two measurements.
Trehaiose solution of the invention contains trehaiose in 0,2 - 68,9 g/dL concentration range, at preferably 40 g/dL dissolved in deionized water or another solution in a manner 25 not to affect trehalase activîty. 1 unit volume of this solution is mixed with 39 units volume urine. In other applications of the invention, if trehaiose solution contains trehaiose at a concentration different from 40 g/dL, solution and urine volumes are changed to contain trehaiose at a final concentration of preferably 1 g/dL in 0,1 - 5 g/dL range. It is kept at an appropriate température for an approprîate time. Trehaiose of the solution is converted 30 into glucose by trehalase enzyme in urine. The higher the trehalase in concentration in urine the more the glucose is produced.
The kit used for measurement of glucose in urine routinely can also measure glucose in urine having been added solution ofthe invention.
Sarre measurement is also mode by use of deionized water added urine of same volume 5 instead of solution and incubated at the same conditions (time and température). Resuit of this measurement is assumed as blank.
The différence between two different urine glucose measurements by solution and deionized water added shows trehalase activity.
From glucose concentration formed by Trehalase enzyme, trehalase activity resuit is calculated in U/L. In the calculation the time period when solution is incubated by urine, dilution factor and final incubation volume are also taken into account. Trehalase activity producing 2 pmol glucose from 1 pmol trehaiose per minute is assumed as one Unit (U).
Urine Trehalase Activity Measurement Example 1:
Collection of Urine Sample:
A random midstream urine was collected from patient. Urine sample should not be cloudy. 20 The urine sample was put into a clean and dry tube. In alternative applications, the samples not to be analyzed immediately and can be stored for 2 hours at +4°C and 48 hours at -20°C in closed tubes.
Mixture and incubation of Urine and 40% trehaiose solution:
975 pL urine taken from patient and 25 pL 40% trehaiose solution were put into Sample tube. 975 pL urine taken from patient and 25 pL deionized water were put into blank tube. Tubes were incubated at 37°C for 30 minutes.
In alternative applications, if trehaiose solution is of different concentration, volumes of used urine and solution can be changed accordingly. Incubation period and température may vary subject to laboratory conditions.
Trehalase Activity Measurement:
Measurement principle is based on measurement of glucose formed by conversion of trehaiose in urine into glucose by trehalase enzyme.
Urine glucose was measured by glucose kit of ARCHITECT brand (Reference no: 3L82, Germany) at Abbot Architect C8000 (USA) device by kinetic colorimétrie method according to kit instructions.
Glucose was measured separately în trehalose solution added urine and deionized water added urine samples and the différence was accepted as trehalase activity.
Principle of Urinary Glucose Measurement Experiment:
Glucose is phosphorylated by hexokinasein presence of adenosine triphosphate (ATR) and magnésium ions; and glucose-6-phosphate (G-6-P) and adenosine diphosphate (ADP) occurs, While glucose 6 phosphate-dehydrogenase (G-6-PDH) oxidizes G-6-P to phosphogluconate, nicotinamide adenine dinucleotide (NAD) is converted to reduced nicotinamide adenine dinucleotide (NADH).One NADH is produced per each consumed glucose molécule. Produced NADH absorbs light at 340 nm and is detected spectrophotometrically as increased absorbance . Method is linear up to < 800 mg/dL (44 mmol/L).
Calculation of Urinary Trehalase Activity:
After separate glucose measurements with trehalose solution added urine and deionized water added urine samples, following results were obtained:
Glucose concentration of Trehalose solution added urine: 115 mg/dL
Glucose concentration of deionized water added urine: 7 mg/dL
Différence = 115 mg/dL- 7 mg/dL= 108 mg/dL= 1080 mg/L= 6mM= 6000 pM (Note: Molecular weightof glucose is 180g/mol)
Trehalase activity producing 2 pmol glucose from 1 pmol trehalose per minute is assumed as one Unit (U). Since incubation time of experiment is 30 minutes, glucose produced in 1 minute:
6000 pM / 30 min. = 200 pM / min, /2= 100 U/L
Since trehalose solution was added in 1 unit volume into 39 units volume of urine before measurement, the resuit is multiplied by “40-39 = 1.025” to correct dilution factor: Urinary trehalase activity: 100 U/L x 1.025 Urinary trehalase activity: 102.5 U/L
Référé n ces
1. Ishihara R, Taketani S, Sasai-Takedatsu M, Adachi Y, Kino M, Furuya A, et al. ELtSA for urinary trehalase with monoclonal antibodies: A technique for assessment of 5 tubuiar damage. Clin Chem. 2000;
2. M. S-T, S. T, N. N, T. F, R. T, T. K. Human trehalase: Characterization, localization, and its increase in urine by rénal proximal tubuiar damage. Nephron. 1996.
3. NAKANO M, IGUCHI A, KURiMOTO H, SAKAMOTO N. Elévation of Urinary Trehalase and Maltase Activities with Maturity-Onset Diabètes Meltitus. J Clin Biochem
Nutr.2011;
4. Skoczyhska A, Martynowicz H, Poreba R, Antonowicz-Juchniewicz J, Sieradzki A, Andrzejak R. Urinary trehalase activity as an indicator of rénal dysfunction in lead smeiters. Med Pr. 2001;
5. Nakano M, Aoshima K, Katoh T, Teranishi H, Kasuya M. Urinary trehalase activity 15 and rénal brush-border damage in inhabitants of a cadmium-polluted area (Jinzu River basin). Toxicol Lett. 1986;
6. Iwata K, Katoh T, Morikawa Y, Aoshima K, Nishijo M, Teranishi H, et al. Urinary trehalase activity as an indicator of kidney injury due to environmental cadmium exposure. Arch Toxicol. 1988;
7. Sasai-Takedatsu M, Kojima T, Taketani S, Ono A, Kitamura N, Kobayashi Y.
Urinary Trehalase Activity Is a Useful Marker of Rénal Proximal Tubuiar Damage in Newborn Infants. Nephron. 1995;
8. Niwa T, Katsuzak T, Yazawa T, Tatemichi N, Emoto Y, Miyazaki T, et al. Urinary Trehalase Activity in Chronic Glomerulonephritis. Nephron. 1993;

Claims (10)

1. A trehalose solution for use together with urinary glucose measurement kits for measurement of urinary trehalase enzyme activity, in biochemical diagnostic field.
2. The solution according to claim 1 and characterized by containing trehalose in 0,2 68,9 g/dL concentration.
3. A urine trehalase measurement kit comprising solution according to claim 1 or claim 2.
4. A method for measurement of trehalase enzyme in urine and characterized by comprising of the following process steps of:
a) Mixing trehalose solution and urine sample,
b) Incubating mixture at a predetermined température and duration,
c) Measurement of glucose in mixture by glucose measurement kit with selected urine,
d) Measurement of glucose in deionized water added urine mixture at said équivalent conditions in previous steps,
e) Evaluation of différence of results between two glucose measurements.
5. The method according to claim 4 and characterized by comprising said trehalose solution in process step “a contains trehalose at 40 g/dL concentration.
6. The method according to claim 4 characterized in that in process step a” 1 unit volume trehalose solution is mixed to 39 unit volume urine.
7. The method according to claim 4 characterized in that in process step d” 1 unit volume deionized water is mixed with 39 unit volume urine.
8. The method according to claim 4 and characterized in that in process step “e, trehalose solution and deionized water are mixed and the différence between two different urinary glucose measurements is calculated as trehalase activity.
9, The method according to claim 4 and characterized in that in process step “e”, from glucose concentration formed by Trehalase enzyme, trehalase activity resuit is calculated as U/L.
10. The method according to claim 4 and characterized in that in process step “e”, 5 Trehalase activity producing 2 pmol glucose from 1 pmol trehalose per minute is assumed
OA1202100539 2020-12-30 2021-11-29 A solution for measurement of Trehalase in urine and measurement method using this solution OA20804A (en)

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Application Number Priority Date Filing Date Title
TR2020/22438 2020-12-30

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OA20804A true OA20804A (en) 2023-05-05

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