Jul 25, 1986 - Refractoriness occurs in many patients receiving multiple platelet transfusions. We used a sensitive. ELISA assay to assess the utility.
From bloodjournal.hematologylibrary.org by guest on June 5, 2013. For personal use only.
1987 70: 23-30
An evaluation of crossmatching, HLA, and ABO matching for platelet transfusions to refractory patients JM Heal, N Blumberg and D Masel
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From bloodjournal.hematologylibrary.org by guest on June 5, 2013. For personal use only.
An
Evaluation
of Crossmatching,
HLA,
Transfusions
Refractoriness platelet assess gle
occurs
the
We
utility
donor
Of the
in 222
posttransfusion, matches
had
of the
matching
outcome. crossmatch grade
10,00O/sL
for
transfusions
of
influences was
BX,
and
plasma compatible,
antibodies. the
INCE THE l960s, platelet become vital to the prophylaxis disorders in patients with leukemia, solid tumors.’ products
bleeding
patients.2
in these
fused
patients
become
refractoriness
to
immunological,5 tion
may
that
has
approach
been
donor
platelets
other
role.6 fruitful
The
appear
to
than
HLA-A,B
because bleeding,
mechanisms.8 the patients coagulopathy,
nologic
factors
survival.
now
are
Such
doubts
are
known
to decrease
platelet
and specific crossmatch for detection of IgG and 1gM
Sensitive
available
‘ These
platelets.9’
tests
platelets
appear
survival
of
platelets. patients
However, many with the previously
in patients
contribute to increased platelet a very small subset of refractory in detail. We developed assay,
and
used
spectively
in typical
any tory
patients, patients
has
been
that does assessment
a
sensitive
it to evaluate refractory
because the preselected
clearly
to with
refrac-
patients.
infection, nonimmu-
recovery
to
studies common has
and
donor
Therefore, only been examined
not exclude any of the potential
We patients benefits
reasoned
did
retro-
Vol 70. No 1 (July).
1987:
pp 23-30
by
and
& Stratton.
and meth-
HLA-A.B
and and
complex
With
our
match
in
ABO some-
or
other
crossmatching
grades
therapy
In
HLA-A,B
of donor
immune
ABO
by Grune
to
plasma
an
ill patients.
crossmatch
destruction
mechanism. transfusion
limited
to patients
remain
some
role-
refractory
tially
Inc.
who
were
alloimmunized
as defined
antibodies.
In addition, matching
we analyzed
because
no
important
the
analysis
role
of HLA-A,B
encompassing
immunologic
factors
and
all
has
these
been
ABO poten-
reported.
METHODS
selection.
Single
HLA-A,B
matched,
unrelated
spectively
against
donor
platelets
individual
recipient
collected were
plasma
in
from a closely
crossmatched
5 1 consecutive
retrorefractory
patients for 316 transfusions. All patients had received RBC products from which leukocytes had not been removed, as well as numerous random donor platelet transfusions. All patients had had at least two previous transfusions of pooled random donor platelet concentrates that failed to yield satisfactory corrected platelet count increments (7,500/zL at I to 4 hours). Lymphocytotoxicity screening
for
formed,
anti-HLA-A,B
but all patients
enzyme-linked
antibodies
was
had detectable
immunosorbent
that
a study
would yield a realistic of crossmatching in
the Hematology
cine,
Department
not
antiplatelet
assay
(ELISA)
routinely
per-
antibody technique.
by our Only
one
sity
of Rochester
Unit ofthe
of Pathology Medical
and
Center,
Department
oflnternal
Laboratory
Medicine,
and
American
Red
MediUniver-
Cross
Blood
Services, Rochester Region, NY. Submitted July 25, 1986; accepted February 5, 1987. Supported in part by Dynatech Laboratories, Chantilly, VA, New York State AIDS Institute (AO-107), and American Red Cross Blood Services, Bethesda, MD. Published and
not exclude
typical clinical practice. It might also provide useful insights into the refractory state that could be missed if the study
Blood,
less
to be mechanisms
related
of that
stable,
current
soluble
platelets
by lymphocytotoxic
antiglobulin
utility of crossmatching in refracon the basis of alloimmunization
demonstrated.9
to the
platelet
From
excluded factors that
crossmatching We
that
contribute
HLA-A,B
1987
were
posttransfusion
enzyme-linked platelet
refracbasis of
reasonable
alloantibodies
consumption. patients
hypothesize
than
appear
are with
value
less
techniques are binding to donor
predict
published mentioned
that
bystander”
to
with
detected
recipient
Patient
is one
some
in question often have fever, and splenomegaly. These
not
of
tory
immunologic
We
vant
primarily
as to whether purely on the
are
predictive
predictive
be considerably there
destruction
but
the
in
followed
independent
that
studies patients,
factor
crossmatch,
having
may
increment
patients.
alloimmuniza-
with
platelet
the
the
important
trans-
matching
in dealing
patients.7 Recently, questions have been raised toriness to platelet transfusion occurs
each
in previous
most
was
demonstrate
crossmatch
antigens
Ia
causes
be
ABO.
data
technique,
the
contained
of multiply
refractory.3’4
factors
an important
5,900
Platelet
platelets,
The
survival
refractory
times
recipient’s
(8,200/zL). and
“innocent
with
plasma
50%
transfusion
play
A/BU
C. Increments
transfusion therapy has and therapy of bleeding aplastic anemia, some
Perhaps
although
for
and
to the
These
ABO ods.
transfusion
for
Masel
platelet
reported of
and
for
predicting
typical
The availability of effective has decreased mortality from
clinically
platelet
the
donor
S
lymphomas, and platelet transfusion
.001).
incompatible
When
but
(P
99#{176}F, sepsis or systemic infection, splenomegaly, consumption coagubopathy, bleeding, or a previous history of autoimmune thrombocytopenia. Determination of these factors was made by the physicians caring for the patient and was documented in the medical record. The presence or absence of these factors was not determined for each individual platelet transfusion. The primary diagnoses were acute nonlymphocytic leukemia (21), solid
tumor
(5),
acute
lymphocytic
leukemia
(4),
chronic
myelogenous leukemia (3), preleukemia lymphoma (2), and other hematological
(3), aplastic anemia (2), conditions such as myebofibrosis, erythroleukemia, multiple myeloma, etc. (1 1 ). Three of the patients were children aged 2 SD above the control means described above. Titers of four randomly selected anti-HLA-A,B antibodies were I to 2 orders of magnitude higher with this k-ELISA technique than by lymphocytotoxicity assays. Titers oftwo anti-Pl” antibodies were 1 to 3 orders
of magnitude
greater
by k-ELISA
than
by complement
fixation techniques or 5’Cr release platelet cytotoxicity methods. Thus, we believe that the technique is probably of similar sensitivity to radioimmune9 or immunofluorescent” methods previously shown to be useful as platelet crossmatches. Although anti-A and -B blood group antibodies are detected by this assay, many patients nonetheless exhibit negative crossmatch results with ABO-incompatible platelets.
All patient plasmas were routinely tested (crossmatched) against four to six randomly selected normal donor platelets at the same time that the crossmatch was performed with the HLA-A,B matched platelets that were transfused. All patients had at least one positive crossmatch incompatibility
during
the course with
several
of these non-HLA-A,B
tests,
with
almost
matched
all showing platelets.
All
matched platelets for transfusion were also crossmatched with two to four normal plasmas. This approach allowed us to detect donor platelets that might have significantly elevated levels of IgG or 1gM. Such platelets yield positive crossmatches even with normal donor plasmas. Donor platelets with elevated platelet-associated IgG (PAIgG) or 1gM occurred very rarely and were excluded from the data reported. Platelets were stored no more than I to 5 days at 4#{176}C prior to crossmatching. Such storage does not alter the level of platelet surface lgG or 1gM, or the binding of plasma IgG or 1gM during a crossmatch (data not shown). Measurement ofPAlgG. PAIgG assay is a technical variant of that described for the detection of plasma anti-platelet antibody.’3 HLA-A,B
From bloodjournal.hematologylibrary.org by guest on June 5, 2013. For personal use only.
PLATELET
TRANSFUSIONS
TO REFRACTORY
25
PATIENTS
PAIgG or soluble IgG standards compete with solid-phase lgG for binding to an alkaline phosphatase-linked anti-IgG antiglobulin reagent. The principle of the assay is that increased concentrations of soluble IgG or PAIgG will compete for anti-IgG and reduce anti-IgG binding to the solid-phase IgG. This assay can reproducibly detect changes of -50 molecules per platelet of lgG. Definitions of HLA and ABO match grades. For HLA, A matches are identical at all four HLA-A,B loci; BU matches are those sharing only two or three HLA-A,B antigens present on recipient cells yet possessing no HLA-A,B antigens that differ from those of the recipient due to being homozygous at one or both HLA-A,B loci; BX matches are those with one donor HLA-A,B antigen differing but cross-reactive with one of those of the recipient; C matches are those in which there is one non-cross-reactive antigen present on the donor cells that differs from those of the recipient. BUX
matches
were
classified
For ABO, identical recipient are of the recipient); which
ABO the
as BX.
transfusions same ABO
are those in which both donor and type (eg, an A donor to an A
“plasma-incompatible”
platelets
do not carry
transfusions antigens
are
incompatible
those
with
microcomputer
(Cupertino,
CA)
and
NCSS
ABO ABO carry A to
chi-square
being
further
addition,
contingency
compared
a three-way
tables,
to each analysis
with
other
individual
with
ofvariance
Apple
software
frequencies
Fisher’s
exact
(ANOVA)
was
test.
In
performed
to assess the independent contributions of crossmatch results, H LAA,B and ABO match grades to platelet count increments, and any interactions
between
these
There
fusion
variables.
the
corrected
The
1gM
was
crossmatches
no clear
and
success
rate
at
1 to
significantly
even
for
crossmatch-negative
(43%).
These 0.03),
(P
patible
and for 0.01).
=
ABO
and
time
data
(Fig
4).
match were
At
these
later
transfusions significantly
matches.
The
degree
significantly posttransfusion,
time
yielded inferior
with
of ABO
was
points,
crossmatch-negative in platelet of A/BU
compatibility
did
increments toward better
was
observed. ofcrossmatching,
these dictive formed and
twothe
matching in predicting and three-way ANOVAS
independent
factors. factor
1 to 4 hours ABO).
and
Crossmatching for corrected HLA
(P
=
.02
that BX
not correlate at
>5 results
hours with match-
count increperformed to
contributions
was the most platelet count
(P
C count and
HLA
platelet were
interactional
posttransfusion matching
examined
increments to those
roles
assess
notable
were
platelets
ments,
platelets
particularly
the relative
ABO
to
transfusions.
identical
posttransfusion
To assess and
not statistiaccording
3)
ABO
ABO-identical ing,
was observed was
(Fig
posttransfusion although a trend
C
v
incom-
for crossmatch-negative
results,
hours
5
trend this
arranged
crossmatch-positive
periods
A/BU
increments arranged crossmatch-negative
but
are shown
of the crossmatch
The match A/BU
for
I . A similar
Corresponding match
.001).
ABO
platelets
v ABO
transfusions,
ofABO
