Description
The
125I-hLH IRMA system provides direct quantitative in vitro
determination of human luteinizing hormone (hLH) in human serum. hLH can
be assayed in the range of 0-150 mIU/ml using 100 µl serum samples. Each
kit contains materials sufficient for 100 assay tubes permitting the
construction of one standard curve and the assay of 42 unknowns in
duplicate.
Introduction
The human luteinizing hormone (lutropin or LH)
is a glycoprotein with a molecular weight of 30000, secreted by the
adenohypophysis. Like other glycoprotein hormones (FSH, TSH and HCG),
hLH contains two different subunits, an a-
and a ß-chain, linked by noncovalent bounds. The primary structures of
the a subunits of hLH and of those mentioned
are virtually identical, whilst their ß subunits are different. The ß
subunits are responsible for the immunological and biological
specificity of these hormones.
The hLH synthesis and release is stimulated by
the hypothalamic gonadotropin releasing hormone (GnRH), whereas the
ovarian steroids secreted from the corpus luteum control further
secretions of hLH by negative feedback.
The measurement of luteinizing hormone
concentrations is an important part of the investigation of disorders of
the hypothalamic-pituitary-gonadal axis. It is recommended to measure
both hLH and hFSH to discriminate between hypothalamic and pituitary
dysfunction.
Principle of method
The technology uses two high affinity
monoclonal antibodies in an immunoradiometric assay (IRMA) system.
The 125I labelled signal-antibody
binds to an epitope of the LH molecule spatially different from that
recognised by the biotin-capture-antibody. The two antibodies react
simultaneously with the antigen present in standards or samples, which
leads to the formation of a capture antibody - antigen - signal antibody
complex, also referred to as a “sandwich”.
During a 2-hour incubation period with shaking
immuno-complex is immobilized to the reactive surface of streptavidin
coated test tubes. Reaction mixture is then discarded, test tubes washed
exhaustively, and the radioactivity is measured in a gamma counter.
The concentration of antigen is directly
proportional to the radioactivity measured in test tubes. By
constructing a calibration curve plotting binding values against a
series of calibrators containing known amount of hLH, the unknown
concentration of luteinizing hormone in patient samples can determined
Contents of the kit
|
1 bottle |
TRACER, ready to use.
21 ml, containing about 740 kBq 125I-anti-hLH and
capture anti-hLH in buffer
with red dye and 0.1% NaN3. |
|
6 vials |
STANDARDS, Ready to use.
1.0 ml per vial, containing 0, 0.4, 2.0, 10, 40, 150 mIU/ml (WHO
2nd IS 80/552 Int.Std.) in human serum with 0.1% NaN3.
See Preparation of reagents |
|
1 vial |
CONTROL SERUM.
Lyophilized human serum with 0.1% NaN3.
The concentration of the control serum is specified in the
quality certificate enclosed. See Preparation of reagents |
|
2 boxes |
COATED TUBE, ready to use.
2X50 reactive test tubes, 12x75 mm, packed in plastic boxes. |
|
1 bottle |
WASH BUFFER CONCENTRATE.
20 ml, containing 0.1% NaN3. See Preparation of
reagents |
|
1 pc |
Quality certificate |
|
1 pc |
Pack leaflet |
Materials, tools and equipment required
Test
tube rack
Precision pipettes with disposable tips (100, 200 and 2000 µl)
Distilled water
Vortex mixer
Shaker
Plastic foil
Gamma counter
Absorbent tissue
Recommended
tools and equipment
Repeating pipettes (e.g. Eppendorf)
Dispenser with 1-L reservoir (instead of the 2 ml pipette)
Specimen collection and storage
Serum
samples can be prepared according to common procedures used routinely in
clinical laboratory practice. Samples can be stored at 2-8 °C if the
assay is carried out within 24 hours, otherwise aliquots should be
prepared and stored deep frozen (-20 °C). Frozen samples should be
thawed and thoroughly mixed before assaying. Repeated freezing and
thawing should be avoided. Do not use lipemic, hemolyzed or turbid
specimens. Samples with a hLH concentration higher than that of the most
concentrated standard should be diluted and reassayed.
Preparation of reagents, storage
Add the
wash buffer concentrate (20 ml) to 700 ml distilled water to obtain 720
ml wash solution. Upon dilution store at 2-8 °C until expiry date.
Add
1000 µl distilled water to the lyophilized control serum. Mix gently
with shaking or vortexing (foaming should be avoided).
Ensure
that complete dissolution is achieved, and allow the solution to
equilibrate at room temperature for at least 20 minutes. Store at -20 °C
until expiry date.
Store
the rest of reagents between 2-8 °C after opening. At this temperature
each reagent is stable until expiry date. The actual expiry date is
given on the package label and in the quality certificate.
CAUTION! Equilibrate all reagents and serum samples to room temperature.
Mix all reagents and samples thoroughly before use. Avoid excessive
foaming.
Assay procedure
(For a quick
guide, refer to Table 1.)
|
1 |
Equilibrate reagents and samples to room temperature
before use. |
|
2 |
Label coated tubes in duplicate for each standard
(S1-S6), control serum and samples. |
|
3 |
Homogenize all reagents and samples by gentle mixing to
avoid foaming. |
|
4 |
Pipette 100 µl of standards, control and samples into the
properly labelled tubes. Use rack to hold the tubes. Do not
touch or scratch the inner bottom of the tubes with pipette tip. |
|
5 |
Pipette 200 µl of tracer into each tube. |
|
6 |
Seal all tubes with a plastic foil. Fix the test tube
rack firmly onto the shaker plate. Turn on the shaker and adjust
an adequate speed such that liquid is constantly rotating or
shaking in each tube. |
|
7 |
Incubate tubes for 2 hours, shaking at room temperature. |
|
8 |
Add 2.0 ml of diluted wash buffer to each tube. Decant
the supernatant from all tubes by the inversion of the rack. In
the upside down position place the rack on an absorbent paper
for 2 minutes. |
|
9 |
Return the tube-rack to an upright position, and repeat
Step 8 two more times. |
|
10 |
Count each tube for at least 60 seconds in a gamma
counter. |
|
11 |
Calculate the LH concentrations of the samples as
described in Calculation of results or use special
software. |
Table 1.
Assay Protocol, Pipetting Guide (all volumes in microliters)
|
Tubes |
Total |
Standard |
Sample |
Control |
|
Standard |
|
100 |
|
|
|
Sample |
|
|
100 |
|
|
Control |
|
|
|
100 |
|
Tracer |
200 |
200 |
200 |
200 |
|
Shake for 2 hours at room temperature |
|
Wash
Buffer |
|
2000 |
2000 |
2000 |
|
Decant the fluid and blot on filter paper |
|
Wash
Buffer |
|
2000 |
2000 |
2000 |
|
Decant the fluid and blot on filter paper |
|
Wash
Buffer |
|
2000 |
2000 |
2000 |
|
Decant the fluid and blot on filter paper |
|
Count radioactivity (60 sec/tube) |
|
Calculate the results |
Table 2.
Typical Assay Data
| |
cpm
1 |
cpm
2 |
cpm
mean |
B / T % |
|
Total |
306942 |
306700 |
306821 |
|
|
S1 |
87 |
104 |
96 |
0.03 |
|
S2 |
699 |
734 |
717 |
0.23 |
|
S3 |
2957 |
2901 |
2929 |
0.95 |
|
S4 |
14065 |
14110 |
14088 |
4.6 |
|
S5 |
54103 |
54115 |
54109 |
17.6 |
|
S6 |
175324 |
175144 |
175234 |
57.1 |
|
C |
11538 |
11337 |
11438 |
3.7 |
Figure 1
A typical standard curve
(Do not use to calculate unknown samples)
Calculation of results
The
calculation is illustrated using representative data. The assay data
collected should be similar to those shown in Table 2.
Calculate the average CPM for each pair of assay tubes. Calculate the
normalized percent binding for each standard, control and sample
respectively by using the following equation:
| |
S2-6 [C, Mx] (cpm) - S1
(cpm) |
|
|
B / T % = |
——————————— |
x 100 |
| |
T (cpm) |
|
Using
semi-logarithmic graph paper plot B/T (%) for each standard versus the
corresponding concentration of LH.
Determine the LH concentration of the unknown samples by interpolation
from the standard curve. Do not extrapolate values beyond the standard
curve range.
Out of
fitting programs applied for computerized data processing logit-log, or
spline fittings can be used. Automated data processing systems are also
available.
Characterization of the assay
Assay
parameters
|
NSB / T |
< 0.05% |
|
Bmax / B0 |
> 1000 |
Sensitivity
A detection
limit of 0.02 mIU/ml has been obtained by assaying 20 replicates of the
zero standard. The sensitivity has been determined as the concentration
corresponding to the sum of the mean cpm and its double standard
deviation.
Hook effect
There is no
high dose “hook effect” up to a hLH concentration of 1000 mIU/ml .
Specificity
No cross
reactivity with hFSH and hTSH can be detected in normal physiological
concentrations.
2 000 mIU/ml hCG gives an apparent 3.5 mIU/ml increase in hLH
concentration.
Precision
4 patient
samples were assayed in 15 replicates to determine intra-assay
precision. Values obtained are shown below.
|
Sample |
Number
of replicates |
Mean
value
mIU/ml |
SD
mIU/ml |
CV
% |
|
1 |
15 |
52.3 |
0.4 |
0.7 |
|
2 |
15 |
29.9 |
0.3 |
1.0 |
|
3 |
15 |
6.6 |
0.1 |
1.4 |
|
4 |
15 |
0.2 |
0.02 |
9.3 |
Reproducibility
To determine
inter-assay precision 4 patient samples were measured in duplicates in
20 independent assays by 2 operators using different kit batches. Values
obtained are shown below.
|
Sample |
Number
of runs |
Mean
value
mIU/ml |
SD
mIU/ml |
CV
% |
|
1 |
15 |
0.2 |
0.03 |
12.1 |
|
2 |
15 |
6.5 |
0.2 |
3.1 |
|
3 |
15 |
29.2 |
0.9 |
3.1 |
|
4 |
15 |
51.8 |
1.4 |
2.8 |
Recovery
Recovery was defined as the measured increase expressed as per cent of
expected increase upon spiking serum samples with known amount of hLH.
The average percent recover for 9 serum pools spiked with hLH at 3
levels was: 98.6 ± 4.3 (mean ± SD).
Expected
Values
|
male: |
|
1.9 - 9.4 mIU/ml |
|
female: |
ovulatory peak |
25 - 94 mIU/ml |
| |
pre- and postovulatory |
0.7 - 9.0 mIU/ml |
| |
postmenopausal |
13 - 80 mIU/ml |
It is
recommended that each laboratory determine a reference range for its own
patient population.
Procedural notes
1)
Source of error! Reactive test tubes packed in plastic
boxes are not marked individually. Care should be taken of not mixing
them with common test tubes. To minimize this risk, never take more
tubes than needed out of plastic box, and put those left after work back
to the box. It is recommended to label assay tubes by a marker pen.
2)
Source of error! To ensure the efficient rotation,
tubes should be firmed tightly inside the test tube rack. Never use a
rack type with open hole. An uneven or incomplete shaking may result in
a poor assay performance.
3)
Addition of wash buffer. For the addition of wash
buffer the use of a common laboratory dispenser equipped with a 1-L
glass bottle, and a flexible outlet tubing end is recommended. In lack
of this tool a large-volume syringe attached to a repeating pipette can
be used.
Additional information
Components from various lots or from kits of different manufacturers
should not be mixed or interchanged.
Precaution
Radioactivity
This product
contains radioactive material. It is the responsibility of the user to
ensure that local regulations or code of practice related to the
handling of radioactive materials are satisfied.
Biohazard
Human blood
products used in the kit have been obtained from healthy human donors.
They were tested individually by using approved methods (EIA, enzyme
immunoassay), and were found to be negative, for the presence of both
Human Immunodeficiency Virus antibody (Anti-HIV-1) and Hepatitis B
surface Antigen (HBsAg).
Care
should always be taken when handling human specimens to be tested with
diagnostic kits. Even if the subject has been tested, no method can
offer complete assurance that Hepatitis B Virus, Human Immunodeficiency
Virus (HIV-1), or other infectious agents are absent. Human blood
samples should therefore be handled as potentially infectious
materials.
Chemical
hazard
Components contain sodium azide as an antimicrobial agent. Dispose of
waste by flushing with copious amount of water to avoid build-up of
explosive metallic azides in copper and lead plumbing. The total azide
present in each pack is 74 mg.
 |
Use by |
 |
In vitro diagnostic medical device |
 |
Control |
 |
Batch code |
 |
Manufacturer |
 |
Standard |
 |
Caution, consult accompanying documents |
 |
Radioactive material |
 |
Coated tube |
 |
Biological risk |
 |
Temperature limitation
Store between 2-8 °C |
 |
Tracer |
 |
Consult instructions for use |
 |
Catalogue number |
 |
Wash buffer |
|
_irma_test_1.htm_cmp_copy-of-sweets000_bnr.gif)
