Thrombocytopenia detected during pregnancy addresses the issue of its mechanism and of the possible occurrence of neonatal thrombocytopenia. To further investigate these issues, 50 women referred to us because of thrombocytopenia detected during pregnancy (platelet count, <150 × 109/L), were extensively studied, as well as their offspring. Among these thrombocytopenic women, we used the threshold of 70 × 109/L to differentiate between mild and severe thrombocytopenia. Whatever the severity of thrombocytopenia, we found biological features of an autoimmune disorder in 48% of the women, and chronic thrombocytopenia in 55%. A familial thrombocytopenia was evidenced in 1 case. These 50 women gave birth to 63 neonates, among whom 24 were thrombocytopenic, either at birth or during the first week of life. Neonatal thrombocytopenia could only be predicted in multiparous women, on the basis of previous neonatal thrombocytopenia in older siblings, and/or when maternal platelet life span study, performed before pregnancy, had evidenced an autoimmune thrombocytopenia (AITP)-like profile. These results suggest that, in case of pregnancy-associated thrombocytopenia, familial and immunological studies, combined with postdelivery iterative platelet counts, should be performed to properly characterize the thrombocytopenia. Moreover, the platelet count of the neonate should be carefully assessed at birth and during the following days, a platelet life span study should be performed after delivery in the mother, because these two parameters are likely to bring valuable information regarding the forthcoming pregnancies and the risk of neonatal thrombocytopenia.

THROMBOCYTOPENIA, observed in about 7% of pregnancies, may be related to previously acquired or inherited diseases or to pregnancy-related complications such as pre-eclampsia, sepsis, or obstetrical disseminated intravascular coagulation.1,2 In 75% of the cases, thrombocytopenia cannot be referred to any of these etiologies. In such cases, pregnancy-associated thrombocytopenia is generally assumed to be secondary to an increased platelet consumption within the placental circulation and/or to hormonal inhibition of megakaryocytopoiesis; it has also been called asymptomatic thrombocytopenia, because it is considered to be devoid of any clinical adverse manifestation in the mother or in the offspring.3,4It has recently been defined as a mild thrombocytopenia that resolves spontaneously after delivery and should not be associated with fetal thrombocytopenia.5 However, several studies have described a fetal and/or neonatal thrombocytopenia occurrence in 4% to 13% of these cases.6,7 The mechanism of neonatal thrombocytopenia is not elucidated so far and addresses the issue of a possible undetected maternal autoimmunity.8 

To assess this hypothesis, we performed an extensive study in a selected population of women referred because of thrombocytopenia detected during pregnancy. We found biological features of an autoimmune disorder in 48% of the women of our series; furthermore, thrombocytopenia persisted after pregnancy in 55% of the women.

Seventy-five women in whom thrombocytopenia (defined as a platelet count <150 × 109/L) had been detected during pregnancy were referred to us by different obstetrical centers. Twenty-five were excluded because information concerning their offspring was lacking or because of loss of follow-up during or after pregnancy. Fifty women who entered the study were investigated either during pregnancy (31 cases) or after delivery (19 cases). At the first visit, they were asked to recall any thrombocytopenic past episode and to bring any platelet count that could have been performed before pregnancy. Women with previous history of autoimmune thrombocytopenia (AITP), systemic lupus erythematosus, or human immunodeficiency virus (HIV) infection were systematically excluded. None exhibited any pregnancy associated complications prone to induce thrombocytopenia, such as sepsis, pre-eclampsia, Hemolysis Elevated Liver Enzymes Low Platelets (HELLP) syndrome, or disseminated intravascular coagulation.1 

Sixty-four neonates were born to these 50 women; 63 of 64 were evaluated, because 1 who died with a Di George syndrome on day 42 was excluded. Platelet counts were performed either at birth, on umbilical cord or peripheral venous blood (50 cases), or during the first week of life (13 cases), depending on local procedures. When neonatal thrombocytopenia, defined as a platelet count less than 150 × 109/L, had been identified, platelet counts were performed until normalization, whereas clinical and biological studies were performed to further define its mechanism.

Immunological tests.

Assessment of platelet-associated IgG (PAIgG) was performed using isotopic methods.9 Circulating or associated antiplatelet autoantibodies were identified by immunocapture assays monoclonal antibody-specific immobilization of platelet antigens (MAIPA test)10 using monoclonal antibodies against platelet glycoproteins (GP) IIb-IIIa, Ib-IX, and Ia-IIa as previously described.8 

Diagnosis of materno-fetal antiplatelet allo-immunization was assessed by identification of parental platelet antigen incompatibility and screening of maternal serum against both a panel of phenotyped donors’ and the father’s platelets.

Serum anticardiolipin antibodies were detected using the enzyme-linked immunoassay described by Harris et al.11 GPL and MPL units were defined as the antibody reactivity of 1 μg/mL of purified anticardiolipin IgG or IgM (kindly provided by E.N. Harris, Louisville, KY). Antinuclear antibodies were detected by indirect immunofluorescence on 4-μm rat liver sections.12Antithyroglobulin antibodies were detected using enzyme-linked immunosorbent assay (ELISA).13 

Isotopic study.

111Indium-labeled autologous or heterologous platelets were infused 2 to 16 months after delivery, after verification of adequate contraception and/or of β human chorionic gonadotrophin (βHCG) level less than 5 IU/L.14 Informed consent was obtained from all patients. Several parameters were studied to define the different patterns of the platelet life span. The mean platelet survival time was calculated using linear and exponential models. Platelet recovery in the circulation was extrapolated from the survival curves to time zero.15 The respective splenic/precordial and hepatic/precordial activity ratios were calculated on platelet infusion (T0), 30 minutes later (T30), and at maximum (Tmax) and plotted on a graph to show early and late distribution of111In-platelets in these organs. A normal platelet life span obtained in 7 healthy volunteers after informed consent had been given was characterized by a mean platelet survival time of 208 hours (range, 192 to 232 hours) and an increment of splenic/precordial sequestration ratio = 1.5 between T30 and Tmax.8 

A thrombocytolysis evocative of AITP also called an AITP-like profile was defined by a mean platelet survival time of less than 130 hours together with a significant secondary increment of the splenic/precordial sequestration ratio, with the value at Tmax being more than 1.5-fold the value of the T30 ratio.16 A profile of hypersplenism was characterized by a mean platelet survival time less than 160 hours, with an immediate increased splenic/precordial sequestration ratio and no further increment after T30.

Statistical analysis.

Mean and standard deviation (SD) values were calculated for each parameter analyzed. χ2-test was used to compare data between groups.

Mothers.

Fifty women who had displayed thrombocytopenia during 63 pregnancies were studied (Tables 1 and2). The mean nadir of the platelet count during pregnancy was 69 × 109/L (SD, 29× 109/L), ranging from 12 to 142 × 109/L. In 26 women (32 of 63 pregnancies), the platelet count was less than 70 × 109/L, with a mean nadir of 46 × 109/L (SD, 14× 109/L). Systematic inquiries disclosed that thrombocytopenia was already present before pregnancy in 4 women (7 pregnancies) in whom it had been incidentally detected, although not further investigated, during a preoperative assessment or a long-term follow-up for Hodgkin’s disease.

No severe bleeding episode was observed during pregnancy; nevertheless, a specific treatment was administered in 22 cases according to the usual procedures applied in the various centers. This treatment had been initiated early in pregnancy in 4 cases or in the prepartum period in 18 cases. It included either high-dose intravenous IgG (IvIgG; 4 cases), oral steroids (10 cases), or platelet transfusion (1 case). IvIgG had been associated with oral steroids in 3 cases. Furthermore, platelet concentrates had been infused in 4 women after unsuccessful IvIgG and/or oral steroid therapy, due to a severe thrombocytopenia in 1 case, before a cesarean section in 2 cases, and in 1 case of hemorrhagic delivery.

Therapy resulted in a complete correction, as defined by a platelet count greater than 150 × 109/L in 5 cases. There was only a partial response in 13 cases, with a 50% increment of the platelet count in 6 cases or an increment ranging from 20% to 50% in 7 cases. In 4 cases, the treatment failed to increase the platelet count.

A long-term follow-up of the platelet count was performed after delivery in 47 women (55 pregnancies). In 26 women (30 pregnancies) thrombocytopenia was actually chronic, as the platelet count remained less than 150 × 109/L long after delivery (from 2 to 36 months), with a mean nadir of 101 × 109/L (range, 35 to 146 × 109/L).

Maternal thrombocytopenia recurred or was aggravated during the subsequent pregnancies in all cases, including all 4 multiparous women whose thrombocytopenia had resolved after the first delivery (Tables 1and 2).

Immunological results are shown in Tables 1 and 2. All of the maternal platelets were sampled for PAIgG (43 during pregnancy). Elevated PAIgG levels (>1,000 IgG/platelet) were observed in 17 cases, 2 of which had received IgG infusion on the days before sampling. It was the only biological abnormality in 7 of 17 cases and was not considered specific. In contrast, a total of 21 women were considered as having biological signs of autoimmunity, because the MAIPA test and/or any other autoantibodies tests resulted positive. Among them, 8 tested iteratively during and after pregnancy were found con- sistently positive. Six were tested only during pregnancy and 7 after delivery. No difference in frequency of detected abnormalities was observed whatever the period of determination (during and/or after pregnancy). A direct MAIPA test, performed in 17 of 50 cases, evidenced an anti–GPIIb-IIIa autoantibody in 4 women with no antiplatelet antibody detected in the serum. An indirect MAIPA test was performed in the serum of 48 of 50 women sampled during pregnancy in 39 cases. A circulating anti–GPIb-IX autoantibody was found in 11 cases. An anticardiolipin antibody (IgM >10 U MPL or IgG >15 U GPL) was found in 7 cases and an antinuclear antibody (>1/50) was found in 2 cases. An antithyroglobulin antibody was detected in 2 cases and was related to an autoimmune thyroiditis in 1 of them.

Conversely, 24 women found negative for both the MAIPA test and anticardiolipin or antinuclear antibodies were considered as not having signs of autoimmunity. Five women were considered as not evaluable because only one of these tests was performed and resulted negative.

Platelet life span was studied in 32 of 50 women within 2 to 16 months after delivery (Table 3). Twenty women were thrombocytopenic at that time, with a platelet count ranging from 11 to 146 × 109/L.

A normal platelet life span was found in only 3 cases. Features of hypersplenism were observed in 9 cases. AITP-like features were found in 18 of 32 cases. Platelet life span features could not be precisely related to any of these patterns in the last 2 cases.

To assess the implications of the severity of thrombocytopenia during pregnancy, two groups of women were constituted according to the platelet count threshold of 70 × 109/L (Table 4): 2 multiparous women had to be excluded because of discordant results in their offspring (see below). Comparing the two groups for maternal and neonatal parameters, there was no difference regarding both the number of mothers diagnosed with chronic thrombocytopenia after pregnancy and the number of thrombocytopenic neonates. Among the 32 evaluated cases, an AITP-like profile was observed in 11 of 17 cases in the group of severe thrombocytopenia as compared with 7 of 14 in the group of mild thrombocytopenia. Surprisingly, biological signs of autoimmunity were found more frequently in the group of mild thrombocytopenia (14 of 22 as compared with 7 of 22; P < .05).

Fetuses and newborns.

Percutaneous umbilical blood sampling was performed in 22 fetuses stemmed from 21 women at gestational ages ranging from 32 to 38 weeks. Whereas no fetal bleeding was observed, fetal bradycardia occurred in 1 case, leading to cesarean section a few hours after sampling. Among the 22 fetuses, 4 disclosed moderate thrombocytopenia, with platelet counts of, respectively, 70, 80, 106, and 115 × 109/L and were delivered without complication, either by cesarean section or by vaginal delivery.

Sixty-three babies were included in the study. Nineteen were born after a cesarean section because of fetal thrombocytopenia, detected by fetal blood sampling in 2 cases, thrombocytopenia observed in the previous siblings in 1 case, maternal thrombocytopenia in 1 case, or an obstetrical reason in 15 cases.

The platelet count was found normal in 39 neonates, which was further confirmed within the first week of life in 25 of them. Thrombocytopenia was found in 24 neonates, either at birth (15 cases) or during the first week of life (9 cases; Table 5). The mean nadir of postnatal platelet count in the 24 thrombocytopenic newborns was 52 × 109/L (range, 13 to 140 × 109/L) and was reached on day 4 (range, 0 to 15 days). Only 1 of the 24 thrombocytopenic newborns displayed hemorrhagic symptoms (petechiae and a scalp hematoma) after a vaginal delivery and was treated by oral steroids (1 mg/kg/d and tapered) until day 69, when the platelet count increased to 80 × 109/L. The platelet count at birth was 75 × 109/L and reached a nadir of 13 × 109/L on day 15.

Treatment with IvIgG (1 g/kg/d ×1 or 0.4 g/kg/d ×5) was performed in 10 cases and resulted in a complete correction in 4 cases or in a transient efficacy in 2 cases. In the 4 remaining cases, data were not available. Thrombocytopenia resolved spontaneously in 2 cases. Evolution was favorable in all cases, with a normalization of platelet count within 11 days (range, 8 to 25 days) in the 8 cases in which it could be assessed.

A nonimmune neonatal pathology that could account for neonatal thrombocytopenia was found in 3 cases: 1 case of neonatal staphylococcus infection, 1 neonatal Rotavirus infection, and 1 intrauterine growth retardation.17 

A parental human platelet antigen incompatibility was found in 5 of the 11 cases in which it was assessed. However, despite the presence of thrombocytopenia in 3 newborns, the diagnosis of maternofetal alloimmunization could not be ascertained, due to the absence of detectable alloantibody in the mother’s serum.

To find out predictors of neonatal thrombocytopenia, two groups of neonates were constituted according to their platelet count and compared regarding siblings’ platelet counts and maternal parameters (Table 6). The offspring of multiparous women were consistently either thrombocytopenic or not thrombocytopenic in 10 of 12 cases. In these 10 cases, we found the platelet count to be normal or decreased in the same proportion in all siblings. This finding supports the hypothesis of the predictive value of this parameter (P < .05), although in a small subset of cases.

Discrepancy in the 2 remaining cases was as follows. In 1 case, neonatal thrombocytopenia in the first-born was most probably related to intrauterine growth retardation (birth weight, 1,980 g in a full-term newborn), whereas the sibling had a normal platelet count both on percutaneous umbilical blood sampling and at birth. In the last case, antenatal platelet count was found within the normal range in each of the 2 successive siblings. However at birth, the firstborn had exhibited a moderate thrombocytopenia with a platelet nadir or day 5, whereas the second one had a persistent normal platelet count up to day 3.

When excluding the 2 cases discussed above, maternal chronic thrombocytopenia was associated with neonatal thrombocytopenia in 11 of 16 women who delivered thrombocytopenic neonates as compared with 14 of 29 who did not (Table 6). An AITP-like profile and neonatal thrombocytopenia in the previous siblings were significantly more frequently associated with the occurrence of neonatal thrombocytopenia (11 of 12 compared with 7 of 19 and 4 of 4 compared with 0 of 6, respectively). Conversely, the occurrence of neonatal thrombocytopenia did not correlate with the severity of the maternal gestational thrombocytopenia.

Thrombocytopenia, when detected during pregnancy, addresses the issue of a possible related autoimmunity. Most of the studies performed hitherto aimed at identifying, among maternal thrombocytopenias, those of immune origin and at defining criteria predictive of severe fetal thrombocytopenia.7 18 However, both specific diagnostic tools of an immune origin of thrombocytopenia in the mother and predictive maternal markers of fetal thrombocytopenia during pregnancy are still missing.

The present work was designed to better understand the mechanisms of maternal thrombocytopenia during pregnancy and its consequences in the offspring in a small subset of thoroughly investigated women. This group of patients referred to a highly specialized center does not reflect the overall population of thrombocytopenic pregnant women. However, the following conclusions can be reached.

(1) Maternal studies when performed in this group of thrombocytopenic women showed asymptomatic autoimmunity in 21 of 44 cases. Whether it can evolve towards a symptomatic autoimmune disorder is yet unknown. The follow-up is less than 5 years in our study, which does not allow any definite conclusion regarding this issue.

However, these results confirm that some pregnancy-associated thrombocytopenia may be of immune origin,3 with a risk of neonatal thrombocytopenia.

(2) The diagnosis of familial thrombocytopenia, easy to achieve, was established in 1 of our 50 cases. It should be systematically searched for before proposing costly and invasive investigations in a pregnant woman with thrombocytopenia, because no maternal or neonatal bleeding complications have ever been reported in most of familial thrombocytopenias (such as May-Hegglin syndrome or Mediterranean thrombocytopenia).19 

(3) Thrombocytopenia detected during pregnancy did not resolve after delivery in 26 of 47 cases, indicating that 55% of them were actually chronic thrombocytopenia incidentally detected during pregnancy rather than pregnancy-associated thrombocytopenia. Moreover, in our hands, the platelet count during pregnancy was not a reliable predictive marker of the evolution of the maternal disease or of the occurrence of neonatal thrombocytopenia: among women with mild thrombocytopenia (platelet count within 70 to 150 × 109/L), 43% delivered thrombocytopenic neonates and 57% had chronic thrombocytopenia. Furthermore, 64% displayed biological signs of autoimmunity and 50% had an AITP-like profile. It should be noted that all 4 women whose thrombocytopenia had been detected before pregnancy displayed an AITP-like profile. The diagnosis of gestational thrombocytopenia, according to the guidelines of George et al,5 could be ascertained after delivery in only 8 of 50 cases. However, among these 8 women, 5 displayed biological signs of autoimmunity, associated in 1 case with an AITP-like profile. Pregnancy-associated thrombocytopenia can therefore be a misleading terminology that should not be used unless platelet count is found to be normal in the months after delivery. The diagnosis of pregnancy-associated thrombocytopenia is impossible to ascertain in primiparous women in the absence of previous platelet count determination. Furthermore, immunological studies should be performed to detect hidden autoimmunity.8 

(4) As previously shown,7,20 we did not find any statistical correlation between the occurrence of neonatal thrombocytopenia and any of the following maternal parameters: platelet count during pregnancy, evaluation of PAIgG, and characterization of circulating and platelet-associated autoantibodies. Furthermore, no difference was observed in the neonates whether or not mothers had received a specific treatment aimed at increasing the platelet count during pregnancy. However, among the 4 women who displayed platelet-associated anti–GPIIb-IIIa autoantibodies, 3 delivered thrombocytopenic newborns. A recent study suggested that circulating anti–GPIIb-IIIa autoantibodies were likely to be more frequently associated with AITP than with gestational thrombocytopenia but could not be conclusive due to the small number of patients.21Likewise, in our study, the question of whether platelet-associated anti–GPIIb-IIIa autoantibody could be associated with hidden autoimmunity remains speculative.

In women found to be thrombocytopenic during pregnancy, we think that a follow-up of platelet count after pregnancy, which has never been extensively achieved,22 would most probably provide some help in evaluating the risk of neonatal thrombocytopenia in subsequent pregnancies. Indeed, the women of our series displaying chronic thrombocytopenia after pregnancy had, to some extent, delivered more frequently thrombocytopenic newborns (11 of 16 v 14 of 29). This might be of interest when the previous siblings’ platelet count is not available.

(5) In contrast, two parameters in multiparous women significantly correlated with the occurrence of neonatal thrombocytopenia. First, the maternal platelet life span, as an AITP-like profile is significantly more often found in the group of women who delivered thrombocytopenic neonates. Unfortunately, it cannot be performed during pregnancy and the results can only be used for subsequent pregnancies. Second is the notion of neonatal thrombocytopenia in a previous sibling. It confirms previous studies showing that, when neonatal thrombocytopenia cannot be ascribed to any recognized cause, its recurrence is likely in the forthcoming siblings.23 

(6) Because of the postnatal decrease of platelet count observed in most cases, severe neonatal thrombocytopenia may be delayed, occurring a few days after birth. This could account for the low incidence of neonatal thrombocytopenia reported in the offspring of thrombocytopenic women when the platelet count is only performed at birth.3,4,18 Moreover, 9 of the 24 thrombocytopenic neonates of our series had a normal platelet count at birth, which suggests that, in the offspring of thrombocytopenic women, the platelet count should be checked not only at birth, but also within days 3 to 5. We found that the nadir of thrombocytopenia was reached later than previously reported.18 This may be due to the cases in which sequential platelet counts were performed only once a week and emphasizes the need of platelet count assessment several times a week in thrombocytopenic neonates until recovery.

Finally, when thrombocytopenia has been detected during pregnancy, whatever the maternal platelet count, and awaiting larger prospective studies based on the overall population of pregnant women to confirm our results, we suggest the following: (1) a familial study should be undertaken, to rule out a familial thrombocytopenia; (2) an immunological study should be performed to detect an asymptomatic maternal autoimmune disorder; (3) the platelet count of the newborn should be performed at birth and repeated twice during the first week of life; (4) iterative maternal platelet counts should be achieved within the 6 months after delivery to detect chronic thrombocytopenia; (5) in our experience, platelet life span study resulted to be of great interest even when platelet count had returned to a normal level, because it led us to detect a compensated thrombocytolysis in a noticeable number of patients; and (6) neonatal thrombocytopenia is most likely to recur in the offspring of a woman who gave birth to a first thrombocytopenic newborn and/or when the maternal life span study is in favor of an AITP-like profile.

The authors thank the physicians who referred their patients from Hôpital Cochin, Hôpital Notre Dame de Bon Secours, Hôpital St Michel, Hôpital St Vincent de Paul, Institut Mutualiste Montsouris, Institut de Puériculture, Paris, France; Hôpital Antoine Béclère, Clamart, France; Hôpital François Quesnay, Mantes la Jolie, France; Hôpital Jean Rostand, Ivry sur Seine, France; Hôpital Louise Michel, Evry, France; Centres Hospitaliers de Compiègne, d’Evreux, de Gonesse, de Neuilly sur Seine, de Saint Cloud, France; and Clinique du Vert Galant, Tremblay en France. The assistance of Monique Dehan in the preparation of the manuscript is gratefully acknowledged.

The publication costs of this article were defrayed in part by page charge payment. This article must therefore be hereby marked “advertisement” in accordance with 18 U.S.C. section 1734 solely to indicate this fact.

1
McCrae
KR
Samuels
P
Schreiber
AD
Pregnancy-associated thrombocytopenia: Pathogenesis and management.
Blood
80
1992
2697
2
Kaplan
C
Forestier
F
Dreyfus
M
Morel-Kopp
MC
Tchernia
G
Maternal thrombocytopenia during pregnancy: Diagnosis and etiology.
Semin Thromb Hemost
21
1995
85
3
Burrows
RF
Kelton
JG
Fetal thrombocytopenia and its relation to maternal thrombocytopenia.
N Engl J Med
329
1993
1463
4
Burrows
RF
Kelton
JG
Incidentally detected thrombocytopenia in healthy mothers and their infants.
N Engl J Med
319
1988
142
5
George
JN
Woolf
SH
Raskob
GE
Wasser
JS
Aledort
LM
Ballem
PJ
Blanchette
VS
Bussel
JB
Cines
DB
Kelton
JG
Lichtin
AE
McMillan
R
Okerbloom
JA
Regan
DH
Warrier
I
Idiopathic thrombocytopenic purpura: A practice guideline developed by explicit methods for the American Society of Haematology.
Blood
88
1996
3
6
Burrows
RF
Kelton
JG
Thrombocytopenia at delivery: A prospective survey of 6175 deliveries.
Am J Obstet Gynecol
162
1990
731
7
Kaplan
C
Daffos
F
Forestier
F
Tertian
G
Catherine
N
Pons
JC
Tchernia
G
Fetal platelet counts in thrombocytopenic pregnancy.
Lancet
336
1990
979
8
Tchernia
G
Morel-Kopp
MC
Yvart
J
Kaplan
C
Neonatal thrombocytopenia and hidden maternal autoimmunity.
Br J Hematol
84
1993
457
9
Muller
JY
Patereaux
C
Doinel
C
Evaluation des IgG fixées sur les plaquettes à l’aide d’un test utilisant une antiglobuline radio-active.
Rev Fran Transfus Immunol Hematol
26
1983
173
10
Kiefel
V
Santoso
S
Weisheit
M
Mueller-Eckhardt
C
Monoclonal antibody-specific immobilization of platelet antigens (MAIPA): A new tool for the identification of platelet-reactive antibodies.
Blood
70
1987
1722
11
Harris
EN
Gharavi
AE
Wasley
GD
Hugues
GRV
Use of an enzyme-linked immunoabsorbent assay and of inhibition studies to distinguish between antibodies to cardiolipin from patients with syphillis or autoimmune disorders.
J Infect Dis
157
1988
23
12
Molden
DP
Nakamura
RM
Tan
EM
Standardization of the immunofluorescent test for autoantibody to nuclear antigens (ANA): Use of reference sera of defined antibody specificity.
Am J Clin Pathol
82
1984
47
13
Bigazzi
PE
Burek
CL
Rose
NR
Antibodies to tissue-specific endocrine, gastrointestinal and neurological antigens
Manual of Clinical Laboratory Immunology.
Rose
NR
Friedman
H
Fakey
JL
1986
764
American Society for Microbiology
Washington, DC
14
ICSH Panel on Diagnostic Applications of Radionuclides
Recommended method for Indium-111 platelet survival studies.
J Nucl Med
29
1988
564
15
Harker
LA
Finch
CA
Thrombokinetics in man.
J Clin Invest
48
1969
963
16
Karpatkin
S
Garg
SK
Siskind
GW
Autoimmune thrombocytopenic purpura in the compensated thrombocytolytic state.
Am J Med
51
1971
1
17
Van den Hof
MC
Nicolaides
KH
Platelet count in normal, small, and anemic fetuses.
Am J Obstet Gynecol
162
1990
735
18
Dreyfus
M
Kaplan
C
Verdy
E
Schlegel
N
Durand-Zaleski
Tchernia
G
the Immune Thrombocytopenia Working Group
Frequency of immune thrombocytopenia in newborns: A prospective study.
Blood
89
1997
4402
19
Goodwin
HA
Grisburg
AD
May-Hegglin anomaly.
N Engl J Med
26
1974
117
20
Hart
D
Duntez
C
Nardi
M
Porges
RF
Weiss
A
Karpatkin
M
An epidemic of maternal thrombocytopenia associated with elevated antiplatelet antibody.
Am J Obstet Gynecol
154
1986
878
21
Lescale
KB
Eddleman
KA
Cines
DB
Samuels
P
Lesser
ML
McFarlaand
JG
Bussel
JB
Antiplatelet antibody testing in thrombocytopenic pregnant women.
Am J Obstet Gynecol
174
1996
1014
22
Brighton
TA
Evans
S
Castaldi
PA
Chesterman
CN
Chong
BH
Prospective evaluation of the clinical usefulness of an antigen-specific assay (MAIPA) in idiopathic thrombocytopenic purpura and other immune thrombocytopenias.
Blood
88
1996
194
23
Christiaens
GCML
Nieuwenhuis
HK
Bussel
JB
Comparison of platelet counts in first and second newborns of mothers with immune thrombocytopenic purpura.
Obstet Gynecol
90
1997
546

Author notes

Address reprint requests to Nadine Ajzenberg, MD, Laboratoire d’Hématologie, Hôpital de Bicêtre, 78 rue du Général Leclerc, 94275 Bicêtre Cedex, France; e-mail: etudba@mailhost.kb.inserm.fr.

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