DOI: 10.1055/s-0040-1713916 - volume 42 - Novembro 2020
Sá, Catherine Primo Nogueira de; Jiménez, Mirela Foresti; Rosa, Marcos Wengrover; Arlindo, Ellen Machado; Ayub, Antonio Celso Koehler; Cardoso, Rodrigo Bernardes; Kreitchmann, Régis; Beitune, Patrícia El
Recent observations support the hypothesis that an imbalance between angiogenic factors has a fundamental role in the pathogenesis of pre-eclampsia and is responsible for the clinical manifestations of the disease. The goal of the present study was to evaluate the sensitivity, specificity, and the best accuracy level of Soluble fms-like tyrosine kinase-1 (sFlt-1), placental growth factor (PlGF), and sFlt-1/PlGF ratio in maternal serum and protein/creatinine ratio in urine sample to define the best cutoff point of these tests to discriminate between the patients with gestational hypertension and the patients with pre-eclampsia, to evaluate the possibility of using them as diagnostic methods.
A prospective longitudinal study was performed, and blood samples were collected from 95 pregnant patients with hypertension to measure serum concentrations of biomarkers sFlt-1 and PlGF. Urine samples were collected for protein screening. Significance was set as p < 0.05.
The sFlt-1/PlGF ratio demonstrated a sensitivity of 57.5% and a specificity of 60% using 50.4 as a cutoff point. The test that showed the best accuracy in the diagnosis of pre-eclampsia was protein/creatinine ratio, with a sensitivity of 78.9% and a specificity of 70% using 0.4 as a cutoff point and showing an area under the receiver operating characteristic curve of 0.80 (p < 0.001).
No studied laboratory test proved to be fairly accurate for the diagnosis of pre-eclampsia, except for the protein/creatinine ratio. The evidence is insufficient to recommend biomarkers sFlt-1 and PlGF to be used for the diagnosis of pre-eclampsia.
The hypertensive disorders of pregnancy are a leading cause of maternal and perinatal mortality and morbidity worldwide, especially in developing countries, affecting 10% of pregnancies, and have been responsible for high costs to the health system.123 Pre-eclampsia and gestational hypertension are characterized by the new onset of hypertension (> 140 mm Hg systolic or > 90 mm Hg diastolic) after 20 weeks of gestation. The next step is to define whether this represents pure gestational hypertension or pre-eclampsia. Pre-eclampsia is diagnosed by hypertension and the coexistence of one or more of the following conditions: proteinuria (urine protein/creatinine > 0.3 mg/mg or > 300 mg/day); maternal organ dysfunction (renal insufficiency, liver involvement, neurological complications, hematological complications); and uteroplacental dysfunction (fetal growth restriction).45 Although often accompanied by new onset proteinuria, hypertension and other signs or symptoms of pre-eclampsia may present in some women in the absence of proteinuria.6
The pathogenesis of pre-eclampsia involves deficient trophoblast invasion that is responsible for altered uterine blood flow and placental oxidative stress.7 Recent observations support the hypothesis that altered expression of placental antiangiogenic factors is responsible for the clinical manifestations of the disease. The damaged placenta produces higher concentrations of Soluble fms-like tyrosine kinase-1 (sFlt-1), a soluble receptor for vascular endothelial growth factor (VEGF) and placental growth factor (PlGF) that is released into the maternal circulation and is involved in endothelial dysfunction.891011 Soluble fms-like tyrosine kinase-1 is an endogenous antiangiogenic protein that is made by the placenta and acts by binding and neutralizing the proangiogenic proteins VEGF and PlGF. Decreased concentrations of the circulating proangiogenic factor PlGF and increased concentrations of the antiangiogenic factor sFlt-1 have been observed in pre-eclamptic patients, suggesting that an imbalance between these factors has a fundamental role in the pathogenesis of pre-eclampsia.121314 Thereby, both sFlt-1 and PlGF have been suggested to be useful for the diagnosis of pre-eclampsia.
The goal of the present study was to evaluate the sensitivity, specificity, and the best accuracy level of sFlt-1, PlGF, sFlt-1/PlGF ratio in maternal serum and protein/creatinine ratio in urine sample to define the best cutoff point of these tests to discriminate between the patients with gestational hypertension and the patients with pre-eclampsia, to evaluate the possibility of using them as diagnostic methods. In addition, we evaluated the degree of association of 24-hour proteinuria with sFlt-1, PlGF, sFlt-1/PlGF ratio and protein/creatinine ratio.
A prospective longitudinal study evaluated 95 pregnant women with hypertension in attendance at prenatal clinics and at the obstetric emergency of a tertiary university hospital in the south of Brazil (Maternidade Mário Totta – Santa Casa de Misericórdia de Porto Alegre, state of Rio Grande do Sul, Brazil) over a period of 12 months (October 2010 to October 2011). All included patients signed an informed consent form. The present study was approved by the Institutional Review Board (CEP UFCSPA 10–628).
The present study included pregnant women after 20 weeks of gestation with systolic blood pressure ≥ 140 mm Hg or diastolic blood pressure ≥ 90 mm Hg, measured according to a standard protocol,1516 and with ≥ 1 occurrences of protein on a dipstick or a protein/creatinine ratio ≥ 40 mg/mmol. These tests were considered screening methods. Thus, patients with positive screening had 24-hour proteinuria collection to confirm or exclude pre-eclampsia, considering this test as the evaluation parameter used in our institution for the diagnosis of the disease. Thereby, the 24-hour proteinuria was used to stratify patients into two groups, gestational hypertension and pre-eclampsia. The 24-hour collection was performed during hospitalization of the patient, under supervision of the nursing staff, following standard procedures established by institutional guidelines, which contributes to more accurate results. We excluded patients with diabetes mellitus and vascular disease prior to the pregnancy or preexisting kidney disease.
Blood samples were collected and serum concentrations of sFlt-1 and PlGF were measured at the time of the diagnosis. The Elecsys (Roche Diagnostics Brazil São Paulo, SP, Brazil) immunoassays for determination of sFlt-1 and PlGF and analysis of blood samples were performed at the central laboratory of the Santa Casa. Clinical information was verified through data collection during hospitalization, searching for maternal and gestational data, risk factors, gestational prognosis (eclampsia and HELLP Syndrome), and other relevant evaluation parameters (hyperuricemia, severe hypertension, proteinuria ≥ 5 g, fetal growth restriction). We made a separate analysis with the primigravida group. In addition, patients were stratified into two groups, early-onset pre-eclampsia (< 34 weeks of gestation) and late-onset pre-eclampsia (≥ 34 weeks of gestation).
The quantitative variables were described by mean and standard deviation (SD), or median and interquartile range (IQR). To compare averages between groups, the t-test was applied. For asymmetric variables, we used the Mann Whitney test. To compare proportions, the chi-squared test or the Fisher exact test was applied. Serum levels of sFlt-1 and PlGF, as well as biochemical parameters, were evaluated for sensitivity, specificity, and the optimal cutoff point by receiver operating characteristic (ROC) curve. The Spearman correlation coefficient (r) was used to evaluate the degree of association between the tests. Sample size was calculated considering an α of 0.05 and a β of 0.20 and setting the null hypothesis in an area under the ROC curve of 0.75. A total of 75 patients were necessary. Statistical analysis was performed using PASW Statistics for Windows, Version 18 (SPSS Inc., Chicago, IL, USA) and the significance level adopted was 0.05.
Table 1 shows maternal and gestational data, risk factors (chronic/preexisting hypertension, pre-eclampsia in a previous pregnancy and family history of pre-eclampsia) and some relevant evaluation parameters (uric acid > 6 mg/dL, systolic blood pressure ≥ 160 mm Hg or diastolic blood pressure ≥ 110 mm Hg, proteinuria > 5 g in 24 hours and fetal growth restriction). Besides, we can observe the screening methods, biomarkers sFlt-1 and PlGF, and 24-hour proteinuria levels. A total of 95 pregnant patients had blood samples collected to measure serum concentrations of biomarkers sFlt-1 and PlGF. One patient has been excluded from the analysis because there was no screening test performed, and another patient has been excluded because there was no registered value of PlGF. Thus, the statistical analysis included 93 pregnant patients with hypertension.
Table 1
Sample characterization of patients included in the study
| Variables* | Total Sample (n = 93) | Pre-eclampsia (n = 73) | Gestational Hypertension (n = 20) | p-value |
|---|---|---|---|---|
| Demographic data | ||||
| Maternal age (years old) | 29.1 ± 7.7 | 29.5 ± 7.7 | 27.9 ± 7.8 | 0.422 |
| Body mass index (kg/m2) | 34.0 ± 6.7 | 34.1 ± 7.1 | 33.3 ± 4.4 | 0.666 |
| Gestational data | ||||
| Gestational age at diagnosis (weeks) | 34.2 ± 4.0 | 34.2 ± 4.4 | 34.1 ± 2.5 | 0.915 |
| Nulliparity | 39 (41.9) | 31 (42.5) | 8 (40.0) | 1.000 |
| Risk factors | ||||
| Chronic/preexisting hypertension | 42 (45.2) | 34 (46.6) | 8 (40.0) | 0.787 |
| Preeclampsia in a previous pregnancy | 6 (6.5) | 5 (6.8) | 1 (5.0) | 1.000 |
| Family history of preeclampsia | 3 (3.2) | 3 (4.1) | 0 (0.0) | 1.000 |
| Evaluation parameters | ||||
| Uric acid ≥ 6 mg/dL | 22 (23.9) | 18 (24.7) | 4 (21.1) | 1.000 |
| Severe blood pressure elevation | 47 (50.5) | 38 (52.1) | 9 (45.0) | 0.759 |
| Proteinuria ≥ 5 g in 24 hours | 1 (1.5) | 1 (2.0) | 0 (0.0) | 1.000 |
| Fetal growth restriction | 12 (12.9) | 8 (11.0) | 4 (20.0) | 0.280 |
| Laboratory tests | ||||
| Protein/creatinine (mg/mmol) | 0.47 (0.36–0.96) | 0.54 (0.41–1.13) | 0.33 (0.24–0.42) | < 0.001 |
| Protein/creatinine ratio ≥ 0.4 | 62 (68.9) | 56 (80.0) | 6 (30.0) | < 0.001 |
| Positive preeclampsia screening | 70 (75.3) | 60 (82.2) | 10 (50.0) | 0.007 |
| 24-hour proteinuria (g) | 0.37 (0.29–0.57) | 0.46 (0.34–0.64) | 0.21 (0.15–0.27) | < 0.001 |
| PlGF (pg/mL) | 100 (62.3–235) | 97.7 (62.3–235) | 119 (56.7–283) | 0.495 |
| sFlt-1 (pg/mL) | 5253 (2649–9071) | 5469 (2703–9375) | 3920 (1613–8574) | 0.169 |
| sFlt-1/PlGF ratio | 55.3 (14.7–113) | 58.7 (16.5–122) | 34.3 (6.5–95.5) | 0.258 |
| Uric acid (mg/dL) | 5.16 ± 1.30 | 5.21 ± 1.30 | 4.97 ± 1.31 | 0.475 |
Abbreviations: P1GF, placental growth factor; sFlt-1, Soluble fms-like tyrosine kinase-1.
*
described by mean ± standard deviation, median (percentiles 25 - 75) or n (%).
Pre-eclampsia was confirmed in 73 patients (78.5%). A total of 29 (39.7%) patients had early-onset pre-eclampsia and 44 (60.3%) had late-onset disease. When evaluating the pre-eclampsia group and the gestational hypertension group, there was no association with nulliparity and no significant difference between early or late-onset pre-eclampsia. Only one patient developed eclampsia and HELLP syndrome (1.1%). Most of the pregnant patients were in the 3rd trimester when they entered in the study, justifying higher values for the body mass index (BMI), which was calculated at the moment the patient was included and not in the beginning of pregnancy.
We analyzed laboratory tests individually and could observe a significant association of protein/creatinine ratio and 24-hour proteinuria with the diagnosis of pre-eclampsia. The biomarkers sFlt-1 and PlGF did not have a good accuracy for disease diagnosis. Demographic and gestational data, risk factors and other evaluation parameters did not have a significant association with pre-eclampsia in our study.
We determined the sensitivity and the specificity for different thresholds of a parameter, defining the best cutoff point for each test. Calculating the area under the ROC curve, we evaluated the performance of the studied tests (Table 2). The sFlt-1/PlGF ratio demonstrated a sensitivity of 57.5% and a specificity of 60% using 50.4 as a cutoff point. The protein/creatinine ratio showed the best sensitivity (78.9%) and specificity (70%) using 0.4 as a cutoff point and was the test with the best accuracy level in pre-eclampsia diagnosis, showing an area under the ROC curve of 0.80 (p < 0.001). In Figs. 1 and 2, the sensitivity, specificity and the area under the ROC curve for the sFlt-1, PlGF, sFlt-1/PlGF ratio and protein/creatinine ratio can be observed.
Table 2
Evaluation of the best cutoff point and the area under the ROC curve of the studied tests for the diagnosis of pre-eclampsia, with their sensitivity and specificity
| Tests | Sensitivity | Specificity | Cutoff point | AUC ROC | 95%CI | p-value |
|---|---|---|---|---|---|---|
| sFlt-1/PlGF | 57.5 | 60.0 | > 50.4 | 0.58 | 0.44–0.73 | 0.258 |
| sFlt-1 | 61.6 | 60.0 | > 4671 | 0.60 | 0.46–0.74 | 0.169 |
| PlGF | 57.5 | 60.0 | < 104.1 | 0.55 | 0.41–0.69 | 0.495 |
| Protein/creatinine | 78.9 | 70.0 | > 0.40 | 0.80 | 0.68–0.92 | < 0.001 |
Abbreviations: AUC, area under the curve; CI, confidence interval; P1GF, placental growth factor; ROC, receiver operating characteristic; sFlt-1, Soluble fms-like tyrosine kinase-1.
Fig. 1
ROC curve of sFlt-1/PlGF ratio (A), sFlt-1 (B) and PlGF (C) in the diagnosis of preeclampsia.
We used Spearman correlation to evaluate the degree of association between 24-hour proteinuria with sFlt-1, PlGF, sFlt-1/PlGF ratio and protein/creatinine ratio. For sFlt-1 (rs= 0.175; p = 0.163), PlGF (rs= - 0.066; p = 0.599) and sFlt-1/PlGF (rs= 0.107; p = 0.396), there was no degree of association. The only test that showed significant association with 24-hour proteinuria was protein/creatinine ratio, with a regular association (rs= 0.403; p = 0.001).
Fig. 2
ROC curve of protein/creatinine ratio in preeclampsia diagnosis.
Several studies have evaluated the role of biochemical markers or a combination of biochemical and biophysical markers in the prediction of pre-eclampsia in the 1st and 2nd trimesters of pregnancy. Clinical, ultrasonographic, and laboratory parameters have been explored during early pregnancy as tools for predicting who will later develop pre-eclampsia. None of these, individually, have sufficient sensitivity and predictive values to be useful clinically, even among women at increased risk.1718192021 Regardless of the parameters used, screening for pre-eclampsia in low-risk women is associated with very low positive predictive values ranging from 8 to 33%.22
The most studied antiangiogenic and proangiogenic markers have been sFlt-1 (soluble receptor for VEGF and PlGF) and PlGF. Studies show that lower concentrations of PlGF and higher concentrations of sFlt-1 during pregnancy confer an increased risk for the subsequent development of pre-eclampsia. Some have noted that maternal serum concentrations of these factors significantly separated healthy pregnant women and women with pre-eclampsia, showing the value of these markers in the prediction of pre-eclampsia and in the differential diagnosis of patients with atypical presentations of the disease. In addition, in high-risk women, the sFlt-1/PlGF ratio is altered prior to pre-eclampsia onset.23242526
Recent studies have evaluated the performance of a newly developed assay for biomarkers PlGF and sFlt-1, which has been studied for the prediction, diagnosis and prognosis of patients with pre-eclampsia. A study conducted by Hagmann et al27 showed that in early onset pre-eclampsia, the sFlt-1/PlGF ratio changes 11 weeks before delivery. Zeisler et al28 observed that a sFlt-1/PlGF ratio < 38 rules out pre-eclampsia, irrespective of gestational age, for at least 1 week. In women with an elevated sFlt-1/PlGF ratio > 85 (early-onset pre-eclampsia) or > 110 (late-onset pre-eclampsia), the diagnosis of pre-eclampsia or placenta related disorders is highly likely. Severely elevated sFlt-1/PlGF ratios (> 655 at < 34 weeks; > 201 at ≥ 34 weeks) are associated closely with the need to deliver within 48 hours.29
Many studies evaluated biomarkers for the prediction of pre-eclampsia. Different from those studies, we evaluated angiogenic factors for the purpose of diagnostic correlation with pre-eclampsia. In a longitudinal prospective study, with adherence to methodological criteria, reviewed in detail, excluding any pregnant woman who could be configured to bias the results analysis, we studied the role of biomarkers PlGF and sFlt-1 in the diagnostic of pre-eclampsia. The present study demonstrated the cutoff point for PlGF (104.1) and for sFlt-1 (4671). Considering these biomarkers, the sFlt-1/PlGF ratio revealed the best association with pre-eclampsia diagnosis using 50.4 as a cutoff point. However, our results showed that sFlt-1, PlGF, and sFlt-1/PlGF ratio did not have good diagnostic accuracy.
Although the literature presents favorable evidence, there are many controversies on the benefits that these biomarkers may provide in the assessment of pre-eclampsia. A study conducted at Cambridge University showed that higher levels of sFlt-1 were not associated with the risk of pre-eclampsia but were associated with a reduced risk of delivery of a small for gestational age infant, spontaneous preterm birth, and stillbirth associated with abruption or growth restriction.30 A case-control study showed that sFlt-1 levels had low capacity to discriminate between healthy patients and pre-eclampsia patients.31 A systematic review accomplished at Oxford University demonstrated that a 3rd trimester increase in sFlt-1 and decrease in PlGF levels were associated with pre-eclampsia, specifically severe disease; however, the authors concluded that the evidence is insufficient to recommend these biomarkers to be used for screening.32
The most reasonable conclusions seem to be that determination of sFlt-1/PlGF ratio can serve as an aid in the diagnosis of hypertensive disorders in pregnancy. The performance of maternal levels of these factors, especially on early onset pre-eclampsia, could be further improved by combining several markers. Combining biomarkers with maternal history, mean blood pressure and uterine artery Doppler achieves a detection rate of ∼ 90% of cases to develop pre-eclampsia.33
Some important considerations of our study are presented below. When our study was initiated, in October 2010, the protein/creatinine ratio was considered a screening method. Thus, pregnant women with positive screening (≥ 1 on dipstick or protein/creatinine ratio ≥ 40 mg/mmol) were considered inclusion criteria of the study, requiring the 24-hour proteinuria collection to define or exclude the diagnosis of pre-eclampsia. We used a cutoff level of 0.4 mg/mg for protein/creatinine ratio according to previous studies performed at our institution, because this cutoff point showed the best accuracy level for pre-eclampsia screening in our pregnant women population. Midrange protein/creatinine ratio (0.3 mg/mg) had poor sensitivity and specificity in our study. In another hospital, located in the same city of our study, they found that hypertensive pregnant women with a protein/creatinine ratio ≥ 0.3 mg/mg had worse maternal and perinatal outcomes than those with a protein/creatinine ratio < 0.3 mg/mg.34 The latest guidelines already consider the use of protein/creatinine ratio as part of criteria for the diagnosis of pre-eclampsia, but many authors and institutions continue to use and consider a full 24-hour urine test for accurate results.35 The existing evidence is not, however, sufficient to determine how the protein/creatinine ratio should be used in clinical practice, owing to the heterogeneity in test accuracy and prevalence across studies.36
We made a separate analysis with the primigravida group to assess the correlation with the diagnosis of pre-eclampsia; however, in our study, there was no association with nulliparity. Besides, patients were stratified into 2 groups, early-onset pre-eclampsia (< 34 weeks of gestation) and late-onset pre-eclampsia (≥ 34 weeks of gestation) and, similarly, there was no significant difference between the groups. Maybe these associations could be observed if we had a larger sample.
Although some criteria are currently no longer considered as severity, when analyzed together, they may have clinical significance. Therefore, we evaluated hyperuricemia, severe hypertension, proteinuria ≥ 5 g and fetal growth restriction as relevant parameters. The evaluation of these parameters did not show a significant difference when comparing pre-eclampsia and gestational hypertension. Twenty-four-hour proteinuria > 5 g has not been considered as a maternal prognosis to indicate pregnancy resolution.6
The BMI was calculated at the entry of the study, not in the beginning of the pregnancy, justifying higher values for this ratio. Furthermore, as the sample comprises hypertensive pregnant women, we could observe higher values for the BMI, since obesity is a risk factor for hypertension. Moreover, in recent decades, there has been an increase in weight in the general population. The growing prevalence of obesity is increasingly recognized as one of the most important risk factors for the development of hypertension.37
Concluding, we can observe that there is considerable heterogeneity among reports. There are differences in the analyte and storage conditions, in the gestational periods selected for blood sampling, and in inclusion and exclusion criteria. Some reports include women with risk factors for pre-eclampsia, whereas others excluded this group; some of the study population was exclusively nulliparous women, whereas all parities were included in others. The evidence is neither strong enough nor sufficient to recommend PlGF and sFlt-1 to be used for pre-eclampsia diagnosis or to screen women at risk to develop the disease. Therefore, the use of proangiogenic and antiangiogenic factors in the assessment of pre-eclampsia is a subject of controversy and is currently under investigation. Prospective studies employing rigorous laboratory and study design criteria are needed to determine the clinical usefulness of these tests.
In summary, in our research, no studied laboratory test proved to be fairly accurate for the diagnosis of pre-eclampsia, except for the protein/creatinine ratio. The evidence is insufficient to recommend sFlt-1 and PlGF to be used for the diagnosis of pre-eclampsia. The identification of biomarkers that can contribute to early detection of pre-eclampsia is essential to apply better surveillance and treatment protocols. Besides, demonstrating the clinical utility of these angiogenic markers could affect the management decisions of the obstetrician, improve health outcomes, and reduce costs to the healthcare system.
We would like to thank Roche Diagnostics Brazil for providing the Elecsys immunoassays for the determination of biomarkers sFlt-1 and PlGF.
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