Using genetics to understand the role of antihypertensive drugs modulating angiotensin-converting enzyme in immune function and inflammation.

AIM: Angiotensin-converting enzyme 2 (ACE 2) is the binding domain for severe acute respiratory syndrome coronavirus (SARS-CoV) and SARSCoV-2. Some antihypertensive drugs affect ACE2 expression or activity (ACE inhibitors and angiotensin II receptor blockers [ARBs]), suggesting use of other hypertensives might be preferable, such as calcium channel blockers (CCBs). Given the limited evidence, the International Society of Hypertension does not support such a policy.
METHODS: We used a Mendelian randomization study to obtain unconfounded associations of antihypertensives, instrumented by published genetic variants in genes regulating target proteins of these drugs, with immune (lymphocyte and neutrophil percentage) and inflammatory (tumour necrosis factor alpha [TNF-α]) markers in the largest available genome-wide association studies.
RESULTS: Genetically predicted effects of ACE inhibitors increased lymphocyte percentage (0.78, 95% confidence interval [CI] 0.35, 1.22), decreased neutrophil percentage (-0.64, 95% CI -1.09, -0.20) and possibly lowered TNF-α (-4.92, 95% CI -8.50, -1.33). CCBs showed a similar pattern for immune function (lymphocyte percentage 0.21, 95% CI 0.05 to 0.36; neutrophil percentage -0.23, 95% CI -0.39 to -0.08) but had no effect on TNF-α, as did potassium-sparing diuretics and aldosterone antagonists, and vasodilator antihypertensives. ARBs and other classes of hypertensives had no effect on immune function or TNF-α.
CONCLUSION: Varying effects of different classes of antihypertensives on immune and inflammatory markers do not suggest antihypertensive use based on their role in ACE2 expression, but instead suggest investigation of the role of antihypertensives in immune function and inflammation might reveal important information that could optimize their use in SARSCoV-2.

What is already known about this subject

There are safety concerns about antihypertensives in SARSCoV‐2 regulating ACE2 expression or activity.

Observationally, the use of ACE inhibitors is not related to higher risk of COVID‐19 events, but might have potential benefits.

These observations have not been confirmed in randomized controlled trials and the relation to immune function and inflammation is unclear.

What this study adds

Using Mendelian randomization in the largest available genome‐wide association studies to obtain uncounfounded associations, our study adds to the limited evidence on the role of antihypertensives in immune function and inflammation by revealing a complex pattern of effects of different classes of antihypertensive drugs.

The observed effect of ACE inhibitors and the null effect of angiotensin II receptor blockers on key markers of immune function and inflammation support the current International Society of Hypertension statement.

Indications of beneficial effects of ACE inhibitors on immune function and inflammation should be investigated.

INTRODUCTION

Angiotensin‐converting enzyme 2 (ACE2) is the binding domain of the severe acute respiratory syndrome coronaviruses (SARS‐CoV) and SARSCoV‐2. A key concern is that ACE inhibitors and angiotensin II receptor blockers (ARBs), commonly used antihypertensives, may increase ACE2 expression or activity, and thereby increase the risk of COVID‐19 infection. Correspondingly, calcium channel blockers (CCBs), which do not affect ACE2 expression or activity, have been proposed as an alternative treatment. In contrast, it has also been suggested that upregulation of ACE2 expression might protect against infection if binding of the coronavirus spike protein to ACE2 leads to ACE2 downregulation, but the mechanism has not been assessed. Given the unclear role of ACE inhibitors and ARBs in infection, the International Society of Hypertension has stated “there is no good evidence to change the use of ACE‐inhibitors or ARBs for the management of raised blood pressure in the context of avoiding or treating COVID‐19 infection”. Consistently, limited evidence from a small observational study suggests patients using ACE inhibitors or ARBs had higher CD3 and CD8 T cell counts. Recent observational studies also show no association of use of ACE inhibitors and ARBs with risk of in‐hospital death in patients with COVID‐19. , , A potential benefit was seen with ACE inhibitor use, but this “may be due to residual confounding” and needs to be confirmed in clinical trials, as well as contextualized by mechanistic insight.

In these circumstances when experimental evidence is lacking from drug testing, Mendelian randomization (MR) provides an alternative approach by exploiting genetic variants, randomly allocated at conception, that mimic drug effects. This study design has been successfully applied to assess the efficacy of several medications. , Published genetic variants corresponding to the effects of a range of antihypertensives exist. , , Here, to be comprehensive we used these genetic variants to assess the effects of a comprehensive range of antihypertensives on key markers of immune function and inflammation related to COVID‐19, ie, lymphocyte percentage, neutrophil percentage and tumour necrosis factor alpha (TNF‐α). Severe COVID‐19 is associated with a major immune inflammatory response with abundant lymphocytes, neutrophils and excess inflammation. Lymphocyte percentage is an established predictor of the severity of COVID‐19, neutrophils are a modulator of immune response. TNF‐α, an amplifier of inflammation, is important in acute inflammatory reactions; anti‐TNF therapy has recently been proposed as a promising COVID‐19 treatment strategy.

METHODS

Study design

We used an MR study to obtain unconfounded associations of the effects of antihypertensive drug use largely from published sources with lymphocyte percentage, neutrophil percentage and TNF‐α. Specifically, we used as instruments published genetic variants predicting the effects of the use of different classes of antihypertensive drugs from genes regulating the drug‐target proteins , which were related to systolic blood pressure (SBP) in the UK Biobank. For ACE inhibitors, we also replicated our findings using genetic variants related both to ACE concentration and to SBP in the UK Biobank as instrument. As we used several different sets of instruments, for ease of comparison of the MR estimates, we used their genetic associations with SBP from the UK Biobank in 361 194 white British as a proxy for their effects on antihypertensives.

Exposure

We obtained genetic instruments predicting the effects of the use of ACE inhibitors, ARBs and CCBs, as well as other classes of antihypertensives, specifically alpha‐adrenoceptor blockers, adrenergic neurone blocking drugs, beta‐adrenoceptor blockers, centrally acting antihypertensive drugs, loop diuretics, potassium sparing diuretics (PSDs) and aldosterone antagonists, renin inhibitors, thiazides and related diuretics, and vasodilator antihypertensives from published sources. , Specifically, these published studies gave the genetic variants regulating the expression of the relevant drug target genes and selected the genetic variants related to SBP in different studies (UK Biobank summary statistics released in 2017 or meta‐analysis of UK Biobank and the International Consortium of Blood Pressure Genome‐wide Association Study [GWAS] ), as summarized in Supporting Information Table S1. We further checked the genetic association of these published single nucleotide polymorphisms (SNPs) with SBP in the latest UK Biobank summary statistics (http://www.nealelab.is/uk-biobank/) in 361 194 white British, adjusted for age, age2, sex, interaction of sex with age, and with age2 and 20 principal components, and kept the SNPs related to SBP in the updated summary statistics. Where several different published genetic predictors of the same drug classes existed, we provide estimates for all sets of predictors. The selection process and the resulting genetic predictors are summarized in Supporting Information Tables S1 and S2. We also looked up these SNPs in Phenoscanner (http://www.phenoscanner.medschl.cam.ac.uk/upload/), a platform with comprehensive genotype‐phenotype associations, to check whether these SNPs are associated with immune function or inflammation biomarkers. For ACE inhibitors, we also used as instruments serum ACE concentration, based on a published study in 4147 participants of European ancestry from the Outcome Reduction with Initial Glargine INtervention (ORIGIN) cohort. Specifically, the study provided 17 SNPs predicting serum ACE. For validity we selected SNPs also related to SBP in the UK Biobank as instrument in the main analysis, and used all these SNPs (if the SNP‐outcome association was available) in sensitivity analysis (Supporting Information Table S2).

Outcomes

Genetic associations with lymphocyte percentage and neutrophil percentage were obtained from UK Biobank summary statistics provided by Neale Lab (http://www.nealelab.is/uk-biobank/). The UK Biobank is a large, ongoing, prospective cohort study with median follow‐up time of 11.1 years. It recruited 502 713 people (intended to be aged 40‐69 years, mean age 56.5 years, 45.6% men) from 2006 to 2010 in England, Scotland and Wales, 94% of self‐reported European ancestry. Here, the genetic associations are based on 361 194 white British (167 020, 46% men), adjusted for age, age2, sex, interaction of sex with age, and with age2 and 20 principal components. Genetic associations with inverse normal transformed TNF‐α concentration were obtained from a large GWAS (n = 24 925) in people of European ancestry, mean age 44.6 years, 55% women, adjusted for age, sex, body mass index and the first ten genetic principal components.

Statistical analysis

MR estimates were based on the SNP‐specific Wald estimates (genetic association with outcome divided by genetic association with the exposure), meta‐analysed using inverse variance weighting with multiplicative random effects, as necessary.

In sensitivity analysis, we used different methods with different assumptions about potential bias from horizontal pleiotropy, including Mendelian randomization pleiotropy residual sum and outlier (MR‐PRESSO), a mode‐based method, and contamination mixture method. MR‐PRESSO is able to identify outliers with potential horizontal pleiotropy amongst multiple genetic variants and provide a corrected estimate after removing these outliers. The mode‐based method assumes the true causal effect is the value taken by the largest number of genetic variants, so it is robust to outliers, but the estimates are generally conservative. The contamination mixture method is similar but less conservative than the mode‐based method. ,

All statistical analyses were conducted using R version 3.6.2 (R Foundation for Statistical Computing, Vienna, Austria), and the R package “MendelianRandomization”.

Ethical approval

All the estimates of genetic associations were taken from publicly available summary statistics, obtained from studies previously collected with informed consent, without any personal information in the study.

RESULTS

Genetic instruments

We used one SNP (rs4968783 in ACE) for ACE inhibitors, one SNP for ARBs (rs118123032 in AGTR1) and 12 SNPs for CCBs scaled to SBP (effect sizes) using UK Biobank summary statistics. We also used one SNP (rs4291 in ACE) for ACE inhibitors and 24 SNPs for CCBs derived based on a GWAS meta‐analysis of the UK Biobank and the International Consortium of Blood Pressure. For the 17 SNPs predicting ACE concentration, two SNPs (and also their proxies) were not available in the UK Biobank, leaving 15 SNPs. Of these only three SNPs were also related to SBP in the UK Biobank and retained. In sensitivity analysis, we used all the 15 SNPs as instruments (Supporting Information Table S2).

For the other classes of antihypertensives, we used eight SNPs in ADRA2A, TH, ADRA1D, ADRA1B and ADRA1A for alpha‐adrenoceptor blockers; three SNPs in ADRA2A and KCNJ1 for adrenergic neurone blocking drugs; 10 SNPs in ADRB1, ADRA1D, ADRB2, ADRA1B, KCNH2, ADRA1A and ADRB3 for beta‐adrenoceptor blockers; six SNPs in ADRA2A, GABRA5, NISCH, GABRA2 and GABRA6 for centrally acting antihypertensive drugs; three SNPs in SLC12A1, SLC12A2 and SLC12A5 for loop diuretics; three SNPs in SCNN1D, SCNN1B and NR3C2 for PSDs and aldosterone antagonists; one SNP in REN for renin inhibitors, seven SNPs in GABRB3, GABRG3, SLC12A1, GABRG1, GABRB2, GABRA6 and CA1 for thiazides and related diuretics; and nine SNPs in NPR1, KCNJ1, PTGIR, PDE5A, EDNRA and CA1 for vasodilator antihypertensives (Supporting Information Table S2). None of the genetic variants are directly related to immune function in Phenoscanner.

Effects on immune and inflammatory markers

The genetically predicted effects of the use of ACE inhibitors and CCBs both increased lymphocyte percentage and decreased neutrophil percentage, with a larger effect size for ACE inhibitors (Table 1). The estimates for ACE inhibitors were robust to using genetic variants predicting ACE concentration (Table 2). The genetically predicted effects of ARBs did not affect lymphocyte percentage or neutrophil percentage (Table 1). The estimates for ACE inhibitors and CCBs were consistent using published genetic variants derived based on the UK Biobank or on the meta‐analysis of the UK Biobank and the International Consortium of Blood Pressure (Table 1). Two other classes of antihypertensives, ie, PSDs and aldosterone antagonists (such as spironolactone) as well as vasodilator antihypertensives (such as ambrisentan), also showed similar effects to ACE inhibitors and CCBs on immune markers, ie, they increased lymphocyte percentage and decreased neutrophil percentage (Table 3).

TABLE 1

Association of antihypertensive drugs with lymphocyte and neutrophil percentage using published genetic variants for ACE inhibitors, ARBs and CCBs in the UK Biobank

Class	Source	#SNPs	Lymphocyte			Neutrophil
			Beta	95% CI	P	Beta	95% CI	P
ACEI	Walker et al 12	1	0.78	0.35, 1.22	5 × 10−4	−0.64	−1.09, −0.20	0.004
	Gill et al 13	1	0.87	0.40, 1.35	3 × 10−4	−0.73	−1.21, −0.25	0.003
ARBs	Walker et al 12	1	−0.61	−1.38, 0.17	0.12	0.69	−0.09, 1.47	0.09
CCBs	Walker et al 12	12	0.21	0.05, 0.36	0.01	−0.23	−0.39, −0.08	0.004
	Gill et al 13	24	0.24	0.16, 0.31	2.7 × 10−9	−0.21	−0.29, −0.13	1.9 × 10−7

Abbreviations: ACEI, angiotensin‐converting enzyme inhibitor; ARB, angiotensin II receptor blocker; CCB, calcium channel blocker; CI, confidence interval; SNP, single nucleotide polymorphism.

TABLE 2

Associations of ACE inhibitors with lymphocyte and neutrophil percentage using ACE SNPs as instrument

Class	Source	#SNPs	Lymphocyte			Neutrophil
			Beta	95% CI	P	Beta	95% CI	P
ACEI	Genetic predictors of ACE 14	3	0.52	0.14, 0.90	0.01	−0.61	−0.99, −0.22	0.002

Abbreviations: ACEI, angiotensin‐converting enzyme inhibitor; CI, confidence interval; SNP, single nucleotide polymorphism.

TABLE 3

Associations of other antihypertensive drugs with lymphocyte and neutrophil percentage using published genetic variants

Class	Source	#SNPs	Lymphocyte			Neutrophil
			Beta	95% CI	P	Beta	95% CI	P
Alpha‐adrenoceptor blockers	Walker et al 12	8	−0.08	−0.28, 0.11	0.41	0.12	−0.09, 0.34	0.27
Adrenergic neurone blockers	Walker et al 12	3	0.46	0.05, 0.87	0.03	−0.24	−0.66, 0.17	0.25
Beta‐adrenoceptor blockers	Walker et al 12	10	0.01	−0.17, 0.19	0.93	−0.01	−0.19, 0.16	0.88
	Gill et al 13	6	0.14	−0.08, 0.37	0.21	−0.04	−0.28, 0.20	0.74
Centrally acting antihypertensives	Walker et al 12	6	0.10	−0.39, 0.59	0.68	0.05	−0.55, 0.65	0.87
Loop diurectics	Walker et al 12	3	0.20	−0.22, 0.63	0.34	−0.16	−0.59, 0.26	0.46
PSDs and aldosterone antagonists	Walker et al 12	3	0.77	0.35, 1.18	3 × 10−4	−0.68	−1.10, −0.26	0.002
Renin inhibitors	Walker et al 12	1	−0.61	−1.63, 0.41	0.24	0.49	−0.55, 1.52	0.36
Thiazides and related diuretics	Walker et al 12	7	0.22	−0.08, 0.52	0.15	−0.19	−0.49, 0.12	0.22
Vasodilator antihypertensives	Walker et al 12	9	0.50	0.04, 0.97	0.03	−0.45	−0.86, −0.03	0.04

Abbreviations: CI, confidence interval; SNP, single nucleotide polymorphism.

Genetically predicted ACE inhibitors may lower TNF‐α (Tables 4 and 5), especially when using genetic variants predicting ACE concentration (Table 5). The estimates were robust to using all the genetic variants predicting ACE concentration and different analysis methods (Supporting Information Tables S3 and S4). CCBs did not clearly affect TNF‐α, and nor did other hypertensives (Table 6). The estimates were robust to different analysis methods (Supporting Information Tables S5 and S6).

TABLE 4

Associations of antihypertensive drugs with TNF‐α using published genetic variants for ACE inhibitors, ARBs and CCBs

Class	Source	TNF‐α
		#SNPs	Beta	95% CI	P
ACEI	Walker et al 12	1	−3.95	−8.40, 0.50	0.08
	Gill et al 13	1	−4.11	−8.94, 0.73	0.10
ARBs	Walker et al 12	1	−2.58	−12.3, 7.11	0.60
CCBs	Walker et al 12	11	0.39	−1.92, 2.70	0.74
	Gill et al 13	24	0.83	0.02, 1.64	0.05

Abbreviations: ACEI, angiotensin‐converting enzyme inhibitor; ARB, angiotensin II receptor blocker; CCB, calcium channel blocker; CI, confidence interval; SNP, single nucleotide polymorphism; TNF‐α, tumour necrosis factor alpha.

TABLE 5

Associations of ACE inhibitors with TNF‐α using ACE SNPs as instrument

Class	Source	TNF‐α
		#SNPs	Beta	95% CI	P
ACEI	Genetic predictors of ACE 14	3	−4.92	−8.50, −1.33	0.007

Abbreviations: ACEI, angiotensin‐converting enzyme inhibitor; CI, confidence interval; SNP, single nucleotide polymorphism; TNF‐α, tumour necrosis factor alpha.

TABLE 6

Associations of other antihypertensive drugs with TNF‐α using published genetic variants

Class	Source	#SNPs	TNF‐α
			Beta	95% CI	P
Alpha‐adrenoceptor blockers	Walker et al 12	8	−0.15	−2.21, 1.92	0.89
Adrenergic neurone blockers	Walker et al 12	3	−2.47	−6.53, 1.58	0.23
Beta‐adrenoceptor blockers	Walker et al 12	10	1.16	−0.62, 2.93	0.20
	Gill et al 13	6	1.46	−0.63, 3.56	0.17
Centrally acting antihypertensives	Walker et al 12	6	−1.09	−4.41, 2.23	0.52
Loop diurectics	Walker et al 12	3	1.30	−2.47, 5.07	0.50
PSDs and aldosterone antagonists	Walker et al 12	3	−0.52	−4.53, 3.49	0.80
Renin inhibitors	Walker et al 12	1	3.97	−6.57, 14.5	0.46
Thiazides and related diuretics	Walker et al 12	7	−1.50	−4.88, 1.88	0.39
Vasodilator antihypertensives	Walker et al 12	9	−0.76	−3.91, 2.40	0.64

Abbreviations: CI, confidence interval; PSD, potassium sparing diuretics; SNP, single nucleotide polymorphism; TNF‐α, tumour necrosis factor alpha.

DISCUSSION

Using genetic proxies for drug effects, we found ACE inhibitors, which increase ACE2 expression, increased lymphocyte percentage, decreased neutrophil percentage and may also lower TNF‐α. CCBs, PSDs and aldosterone antagonists, and vasodilator antihypertensives similarly increased lymphocyte percentage and decreased neutrophil percentage, but were unrelated to TNF‐α. However, other antihypertensives, including ARBs, which also increase ACE2 expression, had no effect on immune markers or inflammation. As such, consistent with the statement from the International Society of Hypertension and previous observational studies, , , our findings do not suggest use of antihypertensive drugs based on their role in ACE2 expression, but do not exclude the possibility of their use based on effects on the immune system.

Lower lymphocyte percentage is predictive of higher severity of COVID‐19 infection. Anti‐TNF drugs have been hypothesized as a potential treatment for COVID‐19 infection. As such, the associations of ACE inhibitors with higher lymphocyte, lower neutrophil and possibly lower TNF‐α are not consistent with the hypothesis that ACE inhibitors impair immune function and increase the risk of infection. Given the complex immune response to COVID‐19 infection, these associations should not be interpreted as a protective role of ACE inhibitors on infection. in vivo experiments suggest ACE inhibitors, such as captopril, do not reduce SARS‐CoV‐2 infection. Effects via modulating the immune reaction have not been assessed. A beneficial association of the use of ACE inhibitors with COVID mortality has been observed in a systematic review and meta‐analysis of observational studies. ACE inhibitors might affect immune function and inflammation via expression of ACE2. However, ARBs, which also affect ACE2 expression, had different effects from ACE inhibitors. The target domain of COVID‐19, ACE2, has high expression in the testes. , Sex hormones modulate immune response and inflammation in animals. Testosterone is generally immunosuppressive, while oestrogen tends to be immune‐promoting. , Genetically predicted testosterone was associated with lower lymphocyte percentage in a recent MR study. Statins, which lower testosterone, have been hypothesized to be protective for COVID‐19 by modulation of NF‐κB, mediated by TNF‐α. Further investigation of these mechanistic pathways might help find a unifying explanation for differences in patterns of COVID‐19 by sex and setting, similar to differences in other hormone‐modulated conditions by setting. ,

Despite consistency across genetic instruments, this study has several limitations. First, MR relies on three assumptions, ie, the genetic instruments are related to the exposure, are not related to potential confounders and the effect of the genetic instrument on the outcome is exclusively through the exposure. To satisfy these assumptions, we used SNPs related to the expression of genes regulating the drug target proteins. We also checked that these SNPs are not directly related to immune function, although we cannot exclude the possibility that unidentified pleiotropic association may exist, which is a common limitation of MR studies. However, we compared the estimates using different SNP selections, which gave consistent findings. Given the possibility of unidentified pleiotropy, we used several different analytic methods that are based on different assumptions. The consistent directions of associations across these methods add confidence to the findings. These methods may differ in precision, for example the estimates from mode‐based methods are generally more conservative than the contamination mixture method, so they are used as sensitivity analysis supplementary to the main analysis. Second, measurement error might exist in the single time‐point assay of lymphocyte percentage, neutrophil percentage and TNF‐α. However, any measurement error should be nondifferential, thus bias towards the null, rather than give positive associations with lymphocyte percentage and inverse associations with neutrophil percentage. Third, the genetic associations with TNF‐α were obtained from a relatively small GWAS, which might explain the wide confidence intervals in the association of ACE inhibitors with TNF‐α. The associations were also adjusted for body mass index, which can cause a bias in some situations, but is unlikely to do so here. The study was also limited by the few large GWAS of immunity, thus replication in other large GWAS when they are available will be worthwhile. Fourth, genetic associations with neutrophil and lymphocyte percentages were taken from the participants of UK Biobank, who are healthier than the general population, so the estimates might be underestimated and the MR estimates may not be applicable to patients with infections. However, the direction of associations should be consistent, which adds to the limited evidence of these antihypertensives in immune function and inflammation. Fifth, the associations in Europeans may not apply to other populations, such as Asians. However, causal effects should be consistent across settings. Sixth, genetic effects might be diluted by compensatory processes or feedback mechanisms. The compensation would be expected to mitigate the genetic effects, thus biasing toward the null, which may explain some null associations such as CCBs and testosterone. The effect sizes of the associations are relatively small, which may not be clinically significant, but a small effect size may still matter for population health, especially for antihypertensive drugs which are commonly used. In addition, MR study is more useful in determining the direction of causation than the magnitude of an effect size, so the effect on immune function and inflammation might not be comparable to the short‐term effect of taking antihypertensive drugs.

From the perspective of clinical practice, our findings do not support the replacement of ACE inhibitors with CCBs because they have similar effects on key markers of immune function, although different effects on inflammation. Our findings suggest a role of ACE inhibitors in immune function and inflammation, but this may not be due to, or at least not totally due to, ACE2 expression because ARBs which also affect ACE2 expression did not affect lymphocyte percentage, neutrophil percentage or TNF‐α. Exploring the underlying pathways, especially the pathways that differ between these antihypertensives, would be worthwhile.

CONCLUSION

The effect of ACE inhibitors and the null effect of ARBs on key markers of immune function and inflammation support the current International Society of Hypertension statement that there is no evidence to indicate the use of antihypertensive drugs based on their role in ACE2 expression. However, concern about the effects of ACE inhibitors on immune function has revealed a complex pattern of effects of different classes of antihypertensive drugs whose elucidation might be relevant to both infectious diseases and optimization of the use of antihypertensives which should be further explored.

COMPETING INTERESTS

There are no competing interests to declare.

CONTRIBUTORS

J.V.Z. generated the idea, conducted the analysis and reported the work described in this article. C.M.S. and G.M.L. reviewed the first draft and suggested important additions to the design and content. All authors reviewed and approved the final version.

Supporting Information Table S1 Sources and selections of genetic predictors for different classes of antihypertensive drugs

Supporting Information Table S2 Genetic predictors for effects of different classes of antihypertensive drugs selected in this study

Supporting Information Table S3 Associations of ACE inhibitors with lymphocyte and neutrophil percentage using genetic variants predicting ACE concentration in Mendelian randomization

Supporting Information Table S4 Associations of ACE inhibitors with TNF‐α using genetic variants predicting ACE concentration in Mendelian randomization

Supporting Information Table S5 Associations of antihypertensive drugs with lymphocyte and neutrophil percentage using different analysis methods in Mendelian randomization

Supporting Information Table S6 Associations of antihypertensive drugs with TNF‐α using different analysis methods in Mendelian randomization

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