Laboratory Procedure Manual: Cd4+ T-Lymphocytes and Cd8 T Cells Whole Blood Tricount Method
Laboratory Procedure Manual: Cd4+ T-Lymphocytes and Cd8 T Cells Whole Blood Tricount Method
Laboratory Procedure Manual: Cd4+ T-Lymphocytes and Cd8 T Cells Whole Blood Tricount Method
Method No.:
Revised:
This document details the Lab Protocol for NHANES 2003–2004 data.
Lab
Number Analyte SAS Label
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CD4+ T-lymphocytes and CD8+ T-cells
NHANES 2003–2004
Human immunodeficiency virus (HIV) infection is characterized by a decrease, and eventually, a depletion of
CD4+ T-lymphocytes (helper T cells). By using immunophenotyping, patient specimens are tested for the
proportion of lymphocytes that are T cells, B cells, natural killer (NK) cells, CD4+ T cells (helper T cells), and
CD8+ T cells (suppressor/inducer T cells). This is done by incubating anti-coagulated whole blood with
monoclonal antibodies to the various cellular antigens that identify specific cell populations (phenotypes), and
then lysing the blood to remove red blood cells. The antibodies are conjugated to fluorescent tags that emit light
of a certain frequency when excited by a laser beam. The specimens are analyzed on a flow cytometer to
determine the proportion of cells of a particular phenotype (that emit light at the right wavelength).
The TruCount method (TriTEST 3-color and MultiTEST 4-color) uses TruCount tubes which contain a lyophilized
pellet containing a known quantity of fluorescent beads. A precise quantity of whole blood is added to the tubes,
and the lymphocytes are stained with TriTEST or MultiTEST monoclonal antibodies (mAb). The absolute count
of a full lymphocyte subset profile (CD3+, CD3+CD4+, CD3+CD8+, CD3-CD19+, CD3-CD16/56+) can be
determined in four tubes with TriTEST and two tubes with MultiTEST by calculating the ratio of region events for
each subset to bead events using the BD Biosciences-developed software, MutltiSET.
2. Safety Precautions
A. FOLLOW UNIVERSAL PRECAUTIONS. Assume that blood and body fluids from all patients are
infectious. Handle all specimens used as controls or reagents at Biosafety Level 2.
B. Wear gloves for handling blood or body fluids. Change gloves when they become contaminated and wash
hands after handling specimens. Do not handle door knobs, telephones, or other community objects while
wearing gloves.
C. Wear protective clothing (lab coat, plastic apron, gown, face shield, etc.) while working with potentially
infectious materials. Leave protective clothing in lab area. Wear closed-toe shoes (no sandals).
D. Use a biological safety cabinet, mechanical pipetting devices when possible, and centrifuge specimens in
safety carriers.
E. Lab work surfaces should be decontaminated with a 10% bleach solution following any spill and at the
completion of work activities. If a vacutainer is broken or blood is spilled, cover with 10% bleach and
plastic-backed absorbent paper or “diaper” and let sit for 10 minutes. Double-glove, wipe up, and dispose
of paper and gloves in an autoclave pan. Use 70% isopropanol for surfaces that might be damaged by
bleach, such as the inside of centrifuges.
F. Dispose of contaminated materials in a plastic bag inside an autoclave pan with at least 2 inches of water.
All liquids should be discarded into bleach equivalent to 10% of the total volume. 12×75 mm tubes with
phenotyping leftover solutions are discarded in a special tube canister or jug with 10% bleach.
G. Personnel should wash their hands after removal of protective clothing and before leaving the laboratory.
H. Do not remove the covers to the flow cytometers when the lasers are on. If instructed to remove the cover
by Becton Dickinson for troubleshooting purposes, turn the power off and unplug the power cord.
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CD4+ T-lymphocytes and CD8+ T-cells
NHANES 2003–2004
3. Procedures for Collecting, Storing, and Handling Specimens; Criteria for Specimen Rejection
A. Enumeration of CD4+ lymphocytes from NHANES 1999-2002 HIV-positive participants and age-
matched controls was performed on cryopreserved whole blood using the method reported by Fiebig et.
al. (11).
B. An appropriate specimen consists of anticoagulated whole blood. Specimens must be collected in EDTA
and processed within 30 hours of draw for Becton Dickinson’s TruCOUNT procedures. The specimens
must meet the following criteria. They must be:
(1) Labeled with the patient’s name or local ID, date of collection, and CDC number (specimen number
or DASH number).
(2) Transported to the lab as soon as possible. They should be shipped by Federal Express or AirBorne
from locations outside Atlanta so that they are received the day after they are drawn and are
temperature controlled to 6°C–39°C.
(3) Processed within 48 hours of draw and preferably within 30 hours of draw for EDTA-anticoagulated
specimens.
C. Several 0.5-ml aliquots of the well-mixed whole blood are made in 2-ml cryovials and stored at –70°C until
the day of testing.
4. Procedures for Microscopic Examinations; Criteria for Rejection of Inadequately Prepared Slides
5. Preparation of Reagents, Calibration (Standards), Controls, and All Other Materials, Equipment and
Instrumentation
A. Reagents
(6) Monoclonals are stored at 4°C–8°C and are stable for the dating period on the label. Freezing
and exposure to light should be avoided. Use undiluted.
(7) Fluorochrome: CD45 PerCP, CD3 FITC, CD4 APC, CD8 PE, CD19 APC, CD16+56 PE.
(8) Fluorescence-activated cell sorter (FACS) lysing solution, 10× (#349202). Dilute the concentrate
1:10 with distilled water to make working lysing solution. Make fresh monthly.
(9) Phosphate-buffered saline (PBS), 0.01 M, pH 7.2 (Formula 4550C)
(10) FACS wash solution: sterile PBS, pH 7.2 with 0.1% sodium azide and 2.0% fetal calf serum.
FACS should be heat-inactivated for 30 min at 56°C and Millipore-filtered. Store and use FACS
wash solution at 4°C for 3 months.
B. Supplies
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CD4+ T-lymphocytes and CD8+ T-cells
NHANES 2003–2004
(2) Dispensing bottles for 2 ml, 300 μl, and 450 μl volumes.
C. Equipment
(5) Centrifuge.
A. FACSComp Procedure
The FACScomp software uses CaliBRITE Beads (plastic micro-pheres) to adjust the FACScan, FACSort,
or FACSCalibur settings for immunophenotyping analysis. The FACSort or FACSCalibur contains sensitive
photoelectric components with variable gain settings. The CaliBRITE Beads are used to ensure that the
instrument provides consistent readings from day to day by adjusting the gain settings and fluorescence
compensation values to standard samples of known light scatter and fluorescent intensity.
On the first screen, enter your initials under Operator ID. Make sure the lot identification for the current
batch of CaliBRITE Beads is correct in the software (matches the bead lot numbers on the insert from the
CaliBRITE box). The suffix letter is important because it tells the software what the minimum signal-to-
noise separation is for that lot. Acquire the unlabeled + APC bead mixture; if “PMT’s” set successfully,
acquire the mixed beads after gently inverting the tube several times to mix. If all tests passed successfully,
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CD4+ T-lymphocytes and CD8+ T-cells
NHANES 2003–2004
print the results. See BD’s FACScomp manual for detailed instructions for performing FACScomp on the
three different flow cytometers.
D. Recording of Results.
The results are recorded in the FACScan, FACSort, or FACSCalibur FACScomp Results logbook and
transferred onto Levy-Jennings plots to monitor instrument performance.
E. Acceptance Criterion
(1) FSC noise should be less than 50. If after eliminating air bubbles and repeating the sensitivity test
with a fresh bead dilution the noise is still over 50, request a service call from BD.
(2) If any of the results when plotted on the Levy-Jennings charts are out of range, make new
dilutions of the beads and run again. One point slightly out of range on one day does not have to
be rejected; but if a trend seems to be developing, a service call may be required.
(1) After FACSComp has been performed successfully, set up the CRBC tube for CRBC calibration. In
a 12×75 mm Falcon #352054 tube, add 1.5 ml of isoton and one drop of well mixed CRBC.
(2) Select the “CRBC Acq.alias” document and “Connect to Cytometer”. Under “Counter” the flow rate
should be 400–1000 events/second. Under Cytometer, select “Instrument Settings” and select the
“CRBC Settings” from the CRBC folder. Under Cytometer, select “Detectors/Amps”. Vortex the
CRBC mixture and acquire. The “mean” bars should be centered over the peaks
(3) Set GeoMean of M1 to predetermined target values found in the Instrument Calibration Log Sheet in
the CRBC Values & Settings Book by raising and lowering voltages FL1, FL2, FL3, and FL4 of the
detectors/amps. Clicking on their respective arrows will adjust the average (target) values [i.e. M1,
M2, M3, M4] accordingly. Mode for FL1, FL2, and FL3 should be set to “Log”. Examples of target
values are: Fl1 = 725, FL2 = 681, FL3 = 644.
(4) Record the adjusted FL1, FL2, FL3, and FL4 voltages and GeoMean values in the Instrument
Calibration Log. Rinse the cytometer with dH2O.
(5) CRBC calibration is useful for monitoring the consistency of settings for research studies.
(1) Remove the cryovials from the –70°C freezer in batches of no more than 10. Make sure to compare
the specimen number or patient ID on the specimen vial to the paperwork (transmittal form, etc.)
Thaw quickly in a 37°C water bath.
(3) CD-Chex will be used as a QC control and frozen whole-blood pool as normal control.
(a) Write the panel and antibody added on the top part of the tube (i.e. 4C-A, 4C-B).
(b) Write the specimen’s assigned lab ID on the lower part of the tube (i.e. A–Z, etc).
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CD4+ T-lymphocytes and CD8+ T-cells
NHANES 2003–2004
(5) Pipette 20 μl of the appropriate antibody into the corresponding labeled tube.
(6) Make sure specimens are well mixed before adding 50 μl (using BD pipette) of frozen whole blood to
the corresponding tube.
(9) Add 450 μl (0.45 ml) of FACS lysing solution found in the cabinet and vortex well.
(11) Add 50 μl of TruCOUNT control beads (from refrigerator) to the CD-Chex tube.
(12) Incubate at room temperature in the dark for at least 15 minutes before acquiring the sample.
Acquire within 2 hours of set-up.
(a) TruCOUNT 3Color-4 tube and 4Color-2 tube LNW panels can be performed using BD MultiSet
software.
(b) Open MultiSET software from the Apple menu and then open appropriate schedule (XXX.sch)
from the CLIA Lab folder on the Desktop. Follow the prompting messages from the program to
proceed.
(d) Make sure to select the appropriate locations for data files, reports, and export document storage.
(e) MultiSET data files are saved in CLIA LAB PROJECTS FOLDER on the DeskTop, then save into
the ICL folder in which a new patient folder with the patient ID and date (e.g. MI9901_120303)
has been designated, and finally save into into a folder named MultiSET. Both the patient and
normal go into this folder.
(f) Make sure the appropriate absolute bead count, reagents, and control bead lot ID’s are filled in
and saved.
(h) Open Cytometer from the Apple menu and make sure the LNW instrument settings file from the
current day’s FACScomp results is selected before clicking the Run Test Command.
(14) Append statistics to the same file created for the project.
(15) Run tests and use Manual Gate for analysis; print report before going to the next sample.
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CD4+ T-lymphocytes and CD8+ T-cells
NHANES 2003–2004
B. Calculations
Calculations for the proportion of lymphocytes that are of particular cell type are determined in the MultiSET
software. This software calculates the proportion of cells that are positive with a particular monoclonal
antibody and reports them in whole numbers. Additionally, the values are automatically corrected for the
purity of lymphocytes inside the gate (% of bright CD45+, CD14- cells of all cells in the gate). All results
reported are corrected for lymphocyte purity. Additional calculations are meant for data quality control.
These include adding the CD3+CD4+ and CD3+CD8+ results to equal the CD3 results (+10%) and
accounting for all of the lymphocytes in the specimen by adding the T, B, and NK cells together to total 90–
110%.
The absolute counts of each subset are calculated automatically by the following formula: absolute CD4 or
CD8 or CD3 Count = (# of target population events / # of bead events collected) × (# of beads per test from
the package insert / test volume of 50 μl).
T cell (CD3+) results are determined from the average of the 4 or 2 CD3 values. T helper/inducer cell values
are from the cells that are positive for both CD3 and CD4 (CD3+CD4+). T cytotoxic/suppressor cell values
are from cells that are positive for both CD3 and CD8 (CD3+CD8+). B cell values are those cells that are
CD19+. NK cells are determined to be negative for CD3 but positive for CD16 and/or CD56 (CD3-
[CD16/56]+).
Results are reported as cells/µl, with a reference range obtained from 129 control donors that were obtained
through the CDC Serum Bank. These donors are composed of adult men and women who were healthy at
the time of blood drawing. Racial composition of this group was mixed. The data set from these donors was
analyzed using SAS and the results for CD3+, CD3+CD4+, and CD3+CD8+ are from a univariate analysis,
with the 5th and 95th percentiles being the low and high values. The values for CD19 and CD3-(CD16/56)+
were log-transformed before univariate analysis was performed.
One hundred and seven samples of this set of control donors were also frozen in aliquots and tested and
analyzed on the same flow cytometer using the BD MultiTest TruCount method. The correlation coefficient
(R) of the fresh whole-blood absolute CD4 counts compared to the frozen whole-blood absolute CD4 counts
was 0.9655, with a slope of 0.92489, intercept of 4.6, and mean bias of –67.2.
If a WBC with differential is available from a hematology complete blood count (CBC), a cross check can be
done on the CD4 count using the CD4 percent from the flow cytometry analysis on frozen whole blood and
the calculated absolute lymphocyte count from the CBC on fresh whole blood using the following formula:
A. A freshly drawn peripheral whole-blood specimen from a healthy donor must be run as a daily quality
control with each run of patients for red blood cell (RBC) lysing control.
B. CD-Chex Plus Normal control (Streck Labs #213326) is run using each antibody for precision of absolute
counts.
When a new batch of reagents (whole-blood control, TruCOUNT controls, TruCOUNT tubes and
antibodies, CaliBRITE beads, etc.) is received, log it in on the appropriate Reagent Record sheet
recording the batch number, lot number, quantity, expiration date, date received, and initials. Mark
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CD4+ T-lymphocytes and CD8+ T-cells
NHANES 2003–2004
the batch number in red on the reagent vial. When a new batch is opened, record the date of first
use, and record the ± expected range of values on the appropriate QC sheet in the TruCOUNT
QA/QC notebook. Place a copy of the package insert in the TruCOUNT 3-Color and 4-Color QA/QC
book. Prior to putting new lots of reagents or kits into use, a lot-to-lot reagent check is performed in
parallel with the current lot in use. These results are recorded on the reagent login sheet. If results of
the new lot are not within 5% of the previous lot, repeat with different specimens; if it is still out of this
range, do not use the new lot.
(2) Setup
(a) Set up the whole-blood control* with the patient samples using the same procedure, reagents,
etc. as the patient samples. Add TruCOUNT bead controls to the whole-blood control according
to the TruCOUNT control procedure. Only one level (high, medium, or low) needs to be used.
(b) Acquire on the flow cytometer in the same manner as the participant samples.
(3) Analysis
(a) Analyze the patient samples and whole-blood control in the appropriate software (MultiSET).
(b) Record the whole-blood control percent and absolute values and the TruCOUNT bead counts on
the appropriate pages and columns for cytometer in the TruCOUNT 3-Color and 4-Color QA/QC
book.
(c) Check to see if the values are within the expected range (±) for that lot number.
(a) If the values of either the whole-blood control or the TruCOUNT control beads are out of the
expected range, vortex and acquire again on the same cytometer. If they are in the expected
range, continue with analysis and reporting of the patient samples.
(b) If the values of either the whole-blood control or the TruCOUNT control beads are still out of the
expected range, set them up again with samples from a fresh vial, acquire on the same
cytometer, and analyze. If they are in the expected range, continue with analysis and reporting of
the patient samples.
(c) If the whole-blood control values are still out of the expected range, acquire the whole-blood
control and the patient samples on the backup cytometer.** If they are in the expected range,
continue with analysis and reporting of the patient samples.
(d) If the whole-blood control values are still out of the expected range, try a new lot number of
control or place a service call to BD Biosciences.
(e) If the patient samples are acquired on more than one cytometer and the percent and absolute
values are essentially the same, the patient results can be reported if there is a problem with the
whole-blood control. Otherwise, the whole-blood control and the TruCOUNT control should be
within the expected range before reporting results.
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CD4+ T-lymphocytes and CD8+ T-cells
NHANES 2003–2004
Follow the directions in Section 9.B.(4) for QC that fail to meet acceptable criteria. If the steps outlined
above do not result in correction of the "out of control" values for QC materials, consult the supervisor for
other appropriate corrective actions. Do not report analytical results for runs not in statistical control.
CD4%: 31–65%
CD4 Absolute: 475–1616 cells /µL
CD8%: 13–42%
CD8 Absolute: 209–924 cells/µ
Specimens are allowed to reach room temperature during preparation. The unused portion of the patient specimen is
returned to the freezer.
14. Alternate Methods for Performing Test of Storing Specimens if Test System Fails
There are no acceptable alternative methods of analysis in the laboratory. If the analytical system fails, the extracted
specimens should be stored at –20°C until the analytical system is restored to functionality.
15. Test Result Reporting System; Protocol for Reporting Critical Calls (If Applicable)
16. Transfer or Referral of Specimens; Procedures for Specimen Accountability and Tracking
The database is used to keep records and track specimens for NHANES 2003–2004. Records, including related
QA/QC data, are maintained for years after completion of the NHANES study. Only numerical identifiers are used
(e.g., case ID numbers). No personal identifiers are available. Residual serum from these analyses are transferred to
the McKesson facility.
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REFERENCES
1. Morbidity and Mortality Weekly Report (MMWR); Guidelines for the performance of CD4+ T cell
determinations in persons with human immunodeficiency virus infection. May 8, 1992, Vo1.41, No.RR-8.
2. Morbidity and Mortality Weekly Report (MMWR). Guidelines for performing single-platform absolute
CD4+ T cell determinations with CD45 gating in persons with human immunodeficiency virus. January
31, 2003, Vo1.52, No.RR-2.
3. National Committee for Clinical Laboratory Standards (NCCLS). Clinical applications of flow cytometry.
Quality assurance and immunophenotyping of peripheral blood lymphocytes. NCCLS H42-T, 1992.
6. National Institutes of Health, National Institute of Allergy and Infectious Diseases, Division of AIDS, Flow
Cytometry Advisory Committee. Guidelines for flow cytometric immunophenotyping, Version 1.0,
January 1993.
7. Nicholson, JKA, Jones, BM, Hubbard, M. CD4 T-lymphocyte determinations on whole-blood specimens
using a single-tube three-color assay. Cytometry. 1993;14:685-689.
8. Nicholson, JKA. Immunophenotyping specimens from HIV-infected persons: laboratory guidelines from
the Centers for Disease Control and Prevention. Cytometry. 1994;18:55-59.
9. Nicholson, JKA, Hubbard, M, Jones, BM. Use of CD45 fluorescence and side-scatter characteristics for
gating lymphocytes when using the whole-blood lysis procedure and flow cytometry. Cytometry.
1996;26:16-21.
10. Nicholson, JKA, Hubbard, M, Dawson, C. Evaluation of stabilized whole-blood control materials for
lymphocyte immunophenotyping. Cytometry. 1999;38:268-273.
11. Fiebig, EW, Johnson, DK, Hirschkorn, DF, Knape, CC, Webster, HK, Lowder, J, Busch, MP.
Lymphocyte subset analysis on frozen whole blood. Cytometry. 1997;29:340-350.
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