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 Table of Contents  
ORIGINAL ARTICLE
Year : 2019  |  Volume : 46  |  Issue : 4  |  Page : 244-250

Study the relationship between vitamin A deficiency, T helper 17, regulatory T cells, and disease activity in patients with systemic lupus erythematosus


Department of Physical Medicine, Rheumatology and Rehabilitation, Faculty of Medicine, Menoufia University, Shebeen El-Kom, Egypt

Date of Submission22-Jan-2019
Date of Acceptance17-Apr-2019
Date of Web Publication01-Oct-2019

Correspondence Address:
Dalia S Saif
Lecturer of Physical Medicine, Rheumatology and Rehabilitation Faculty of Medicine-Menoufyia University (MD), 18 El-Maamoon Street, Shebeen El-Kom, Menoufyia Governorate, 32511
Egypt
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Source of Support: None, Conflict of Interest: None


DOI: 10.4103/err.err_5_19

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  Abstract 


Background Systemic lupus erythematosus (SLE) is a complex autoimmune disease with activation of the innate and adaptive immune systems. Vitamin A deficiency causes imbalance of T helper 17 (Th17) and regulatory T cell (Treg), deteriorating the progression of SLE.
Aim To determine the relationship between vitamin A levels and Th17 and Treg level in patients with SLE and its relation to disease activity.
Patients and methods A total of 45 female patients with SLE diagnosed according to the American College of Rheumatology criteria and 45 healthy age-matched and sex-matched patients as control group were included. Full assessment was done including medications, clinical examination (pain evaluation by visual analogue scale and assessment of disease activity by SLE disease activity index), laboratory investigations, and albumin–creatinine ratio. Serum levels of vitamin A were measured by a human KAMIYA kits, and flow cytometry was used for measuring Th17 and Treg percentages.
Results There was a significant deficiency of vitamin A level in patients with SLE compared with controls (P=0.001). There was a significant negative correlation between vitamin A and Th17 (P=0.001) and positive correlation between vitamin A and Treg percentages (P=0.001). There was a negative correlation between vitamin A levels and albumin–creatinine ratio in patients with SLE (R=−0.255). A positive correlation between serum levels of vitamin A and C3 and C4 was found (P=0.001).
Conclusion Vitamin A deficiency is a bad prognostic factor in patients with SLE, affecting Th17/Treg balance. Routine use of retinoic acid may be a promising supplementary agent in patients with SLE, improving its prognosis.

Keywords: systemic lupus erythematosus, Th17/Treg balance, vitamin A


How to cite this article:
Fettouh DS, Saif DS, El Gazzar SF, Sonbol AA. Study the relationship between vitamin A deficiency, T helper 17, regulatory T cells, and disease activity in patients with systemic lupus erythematosus. Egypt Rheumatol Rehabil 2019;46:244-50

How to cite this URL:
Fettouh DS, Saif DS, El Gazzar SF, Sonbol AA. Study the relationship between vitamin A deficiency, T helper 17, regulatory T cells, and disease activity in patients with systemic lupus erythematosus. Egypt Rheumatol Rehabil [serial online] 2019 [cited 2024 Mar 28];46:244-50. Available from: http://www.err.eg.net/text.asp?2019/46/4/244/268444




  Introduction Top


Systemic lupus erythematosus (SLE) is a complex autoimmune disease in which activation of the innate immune system with activation of T and B lymphocytes and autoantibodies production, immune complex deposition, and complement-induced tissue damage occurs. It is characterized with relapsing-remitting course, which occurs at any age, but it has poorer outcome in childhood than adult patients. Its manifestations vary from mild muco-cutaneous to severe life-threatening illness [1].

Pathogenesis of SLE is still unclear, but balance between T helper 17 (Th17) and regulatory T cells (Tregs) underlies the outcome of the disease [2]. The Tregs, a subset of CD4+T cells, are the main regulators of immune response and suppress inflammatory T-cell responses. Th17, a newly discovered subset of CD4+ T cells, is identified according to its ability to produce interleukin (IL)-17A, IL-17F, and IL-22. It has been shown that there is a positive correlation between the number of Th17 and organ damage, whereas there is a negative correlation between Treg and flares in patients with SLE. Thus, the balance between the two cells can be a new therapeutic option in patients with SLE [3].

The cytokines produced by the activated immune system in patients with SLE also suppress the generation of natural Treg cells and promote a proinflammatory T-cell response dominated by Th17 cells [4].

The active metabolite of vitamin A (retinoic acid) has various biologic properties, including its important role in modulating Th17 and Treg balance, as it has the ability to decrease proliferation and IL-6 induction of Th17 while promote the proliferation of Treg; moreover, it enhances transforming growth factor-β signaling in Treg by increasing the phosphorylation of Smad3 [5].

So the use of vitamin A and retinoic acid may be a promising supplementary agent regulating the balance of Th17 and Treg [5].

The aim of this study was to determine the correlation between vitamin A levels and Th17 and Treg populations in patients with SLE and its relation to disease activity.


  Patients and methods Top


This hospital-based case–control study was conducted on 45 female patients with SLE recruited from the outpatient clinic of Rheumatology, Physical Medicine and Rehabilitation department, Menoufia University, between August 2017 and October 2018. All patients fulfilled at least four criteria of the updated American College of Rheumatology criteria [6] with age between 23 and 55 years, presented with active disease, characterized by systemic lupus erythematosus disease activity index (SLEDAI) score more than 3 [7] and did not take vitamin A supplementation. Moreover, 45 healthy age-matched and sex-matched controls and who did not take vitamin A supplementation were recruited. Patients with severe infection or immunodeficiency, patients with features of vitamin A deficiency, and patients with thyroid abnormalities, chronic liver, or renal disease were excluded from this study.

The ethical committee guidelines in Menoufia University were followed, and informed consent was taken from each patient of the study. Full history taking; general examination; local joint examination, with pain evaluation using visual analogue scale [8]; and laboratory investigations, including complete blood count, erythrocyte sedimentation rate, renal function tests (serum creatinine and blood urea), liver enzymes (alanine aminotransferase and aspartate aminotransferase), C-reactive protein (high sensitive), albumin–creatinine ratio, antinuclear antibody, anti-double stranded DNA titer (anti-dsDNA), and C3 and C4 were done. SLEDAI was used to assess the disease activity [7]. Measurement of the serum vitamin A level was done using the vitamin A human KAMIYA biomedical company kits, and flow cytometry also was done for measuring Th17 and Treg percentages [9].

Overall, 15 ml of blood sample was collected from each individual under aseptic conditions. It was divided into three parts: (a) 8 ml was added to EDTA-contained sterile tubes for the determination of complete blood count and CD markers;(b) 5.4 ml was added to sterile plain tubes for assessment of vitamin A level, C-reactive protein, and serum creatinine; and (c) 1.6 ml of blood was delivered into a tube containing 0.4 ml trisodium citrate for erythrocyte sedimentation rate.

The concentrations of serum vitamin A were determined by enzyme-linked immunosorbent assay. A quantitative sandwich enzyme immunoassay technique that measures human vitamin A was used. Standards and samples were sandwiched by the immobilized antibody and biotinylated polyclonal antibody specific for vitamin A, which was recognized by a streptavidin–peroxidase conjugate. All unbound material was then washed away, and a peroxidase enzyme substrate was added. The color development was stopped, and the intensity of the color was measured [10].

Peripheral blood mononuclear cells were isolated from 8 ml of whole blood samples. Blood was mixed with an equal volume of PBS (pH: 7.4), layered on Ficoll reagent (1077 g/ml), and centrifuged at 1800g for 20 min. The buffy coat containing mononuclear cells was recovered, mixed with 20 ml PBS, and centrifuged at 3000g for 10 min, and then the supernatant was discarded. Washed cells were incubated with labeled monoclonal antibody which binds to cells expressing the antibody of interest and then the cells expressing monoclonal were fluorescently stained.

For each sample, three tubes were prepared, one for the unstained sample (auto control), and 100 ml of peripheral blood mononuclear cells at 5×105/tube WAS stained in two tubes: one for Treg with PE-anti-CD4 plus anti-CD25 FITC (fluorescein isothiocyanate) and the other with PE-anti-CD4 for 30 min. Then in both tubes, cells were fixed followed by intracellular staining with PerCP-anti-FoxP3 in first tube and anti-IL17 FITC in the second tube. After incubation for 30 min at 4°C and subsequently washing twice with PBS, the cells were suspended in 300 μl of PBS for final flow cytometry analysis. The percentages of Treg (CD4+CD25+FoxP3+) and T helper 17 (CD4+ anti-IL17+) cells in all samples were determined by flow cytometry, using FACS Calibur flow cytometer (BD Immune Cytometry System, San Jose, California, USA).

Statistical analysis

Data were described as mean±SD. SPSS version 17.0 (IBM Corporation, Chicago, USA) for Windows was used for statistical analysis and generation of graphs. t-Test and Pearson correlation were used [11].


  Results Top


A total of 45 female patients with SLE with a mean age of 36.6 years (range: 23–55) and 45 healthy age-matched and sex-matched controls with a mean age of 34.36 years were included in this study ([Figure 1]).
Figure 1 Showed be corrected to SLEDAI among SLE patients with hypovitaminosis A ad SLE patients with normal vitamin A level.

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Hypovitaminosis A was considered if up to 30 mcg/dl. It was observed in 35 patients with SLE (77.77%) and was normal in all the control group. Vitamin A levels in the patients with SLE were significantly lower compared with controls (P=0.001; [Table 1]).
Table 1 Vitamin A level and age of patients with systemic lupus erythematosus and control group

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There was a significant increase in SLEDAI in patients with SLE with low vitamin A levels compared with those with normal vitamin A levels (P=0.001; [Table 2] and [Figure 2]).
Table 2 Systemic lupus erythematosus disease activity index in patients with systemic lupus erythematosus with low vitamin A level and those with normal vitamin A level

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Figure 2 Shows age and vitamin A level among patients with SLE and control. SLE, systemic lupus erythematosus.

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The was a statistically significant negative correlation between vitamin A level and Th17 level (P=0.001, R=−0.852) and a significant positive correlation between vitamin A and Treg populations (P=0.001, R=0.882; [Table 3] and Graphs 1 and 2.
Table 3 Correlation of vitamin A levels with T helper 17 and regulatory T cell percentages and C3, C4, anti-double stranded DNA titer and albumin–creatinine ratio in patients with systemic lupus erythematosus

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A statistically significant positive correlation between vitamin A and C3 and C4 (P=0.001, R=0.642, and R=0.778) was found, with a negative correlation between vitamin A levels and albumin–creatinine ratio in patients with SLE. Moreover, there was a statistically significant negative correlation between vitamin A and anti-dsDNA titers (P=0.001, R=−0.708; [Table 3] and [Figure 3] and Graph 3.
Figure 3 Shows Treg, Th17, anti-dsDNA, C3, C4, and albumin–creatinine ratio among patients with SLE and control. anti-dsDNA, anti-double stranded DNA; SLE, systemic lupus erythematosus; Th17, T helper 17; Treg, regulatory T cell.

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There were statistically significant differences between patients with SLE with hypovitaminosis A compared with those with normal vitamin A level regarding C3, C4, Treg17, Th17, anti-dsDNA titer, and albumin percent (P=0.001; [Table 4]).
Table 4 Comparison between patients with SLE with hypovitaminosis A with those with normal vitamin A level regarding C3, C4, regulatory T cell 17, T helper 17, anti-double stranded DNA titer, and albumin–creatinine ratio

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  Discussion Top


SLE is a multisystem autoimmune disease that causes persistent inflammation and multiple organ damage. SLE is initiated by imbalance of Th17 and Treg populations [2]. Recent studies showed that increase number of Th17 and reduction of Treg were strongly associated with organ damage and clinical symptoms of SLE [12]. Vitamin A has a major role in immune system regulation especially Th17 and Treg balance [5].

This study showed a significant increase for the incidence of hypovitaminosis A in patients with SLE compared with healthy controls (P=0.001). This comes in agreement with Kida et al. [13] who reported decreased vitamin A levels in patients with SLE. This significant low level of vitamin A is explained by the chronic inflammatory conditions, which decrease the expression of the lecithin retinol acyltransferase enzyme causing disruption of vitamin A storage in the liver.

D’Ambrosio et al. [14] also reported low levels of vitamin A in patients with SLE compared with healthy controls. They explained that by the interference of lecithin retinol acetyl-transferees gene, which may be associated with vitamin A deficiency.

This study showed that the patients with low vitamin A levels have higher disease activity (SLEDAI). This comes in agreement with Hanly et al. [15] as they reported high disease activity in vitamin A-deficient patients as compared with those with normal vitamin A levels due to immuno-regulatory imbalance which caused by vitamin A deficiency.

This study reported the association between vitamin A deficiency and high titer of Th17, albumin creatinine ratio, and anti-dsDNA titer (P=0.001). Moreover, vitamin A deficiency is associated with low titer of Treg, C3, and C4 (P=0.001).

In accordance to our study, Elias and his colleagues reported the significant positive correlation between vitamin A and Treg and negative correlation between vitamin A and Th17. This is owing to the ability of ATRA and other agonists of the retinoic acid receptor alpha (RARα) to inhibit the formation of Th17 cells and promote Treg differentiation [16].

Our results also come in agreement with Nolting et al. [17] and Sobel et al. [18] who reported the significant positive correlation between Treg and vitamin A levels and the negative correlation between it and Th17. They reported that vitamin A can enhance the conversion of naive T cells into Treg and also inhibit Th17 differentiation by inhibiting IL-6 and IL-23 receptor expression.

The negative correlation between serum vitamin A levels and albumin–creatinine ratio in patients with SLE (P=0.091, R=−0.255) was supported by Bennet et al. [19] who reported the high levels of albumin–creatinine ratio when vitamin A decreases.

A significant negative correlation between vitamin A levels and anti-dsDNA titer was reported in our study, which is reported also by Hanly et al. [15].

The significant positive correlation between vitamin A deficiency and low levels of C3 and C4 in patients with high disease activity in our study was supported by Hanly et al. [15], who reported the association between vitamin A- deficiency and complement consumption and low complement levels in SLE patients with high disease activity.

Our study reported a significant increase in Th17 and decrease in Treg in patients with SLE with low vitamin A levels compared with those with normal vitamin A levels (P=0.001). This comes in agreement with Pan et al. [12].

Szmyrka-Kaczmarek et al. [2] reported high Th17 and low Treg levels in vitamin A-deficient SLE patients compared to those with normal vitamin A level. Low level of Treg caused increase autoantibodies productions, tissue damages, and clinical deteriorations in patients with SLE.

In contrast, Yang et al. [20] reported the elevation of both Th17 and Treg populations in patients with SLE. The increased Treg may be a compensatory mechanism to autoimmune processes, such as increase Th17 subset. In this study, we excluded patients with immunodeficiency or those associated with other autoimmune disorders, and our patient groups were larger.

This study also reported significant decreased of C3 and C4 level in vitamin A-deficient patients compared with those with normal levels (P=0.001). This is owing to high disease activity in vitamin A-deficient patients and more complement activation causing decreased C3 and C4. Szmyrka-Kaczmarek et al. [2] reported this decrease in C3 and C4 in patients with active SLE.

In vitamin A-deficient patients, the albumin–creatinine ratio (>30 mg albumin/creatinine) and anti-dsDNA titer were high than patients with normal levels. This proves the severity of organ damage especially the kidneys in vitamin A-deficient patients with SLE owing to immune disruption, autoantibodies production, and immune complex deposition. Bennet et al. [19] reported the same results.


  Conclusion Top


Vitamin A deficiency is a bad prognostic factor in patients with SLE, affecting Th17/Treg balance, as it can inhibit Th17 differentiation and enhance Treg differentiation. Treatment with vitamin A is a promising supplementary option and may provide improvement in SLE prognosis.

Financial support and sponsorship

Nil.

Conflicts of interest

There are no conflicts of interest.



 
  References Top

1.
Joo YB, Park CSY, Won S, Bae S, Danilenko DM, Valdez P. Differences in clinical features and mortality between childhood-onset and adult-onset systemic lupus erythematosus: a prospective single-center study. J Rheumatol 2016; 43:1490–1497.  Back to cited text no. 1
    
2.
Szmyrka-Kaczmarek M, Kosmaczewska A, Ciszak L, Szeteblich A, Wiland P, Hakim R. Peripheral blood Th17/Treg imbalance in patients with low-active systemic lupus erythematosus. Postepy Hig Med Dosw 2014; 68:893–898.  Back to cited text no. 2
    
3.
Lu L, Barbi J, Pan F, Daniel C, Reuter S, Steulten C. The regulation of immune tolerance by FOXP3. Nat Rev Immunol 2017; 17:703–717.  Back to cited text no. 3
    
4.
Valencia X, Yarboro C, Illei G, Lipsky PE, Yarboro C, Illei G. Deficient CD4,CD25 high T regulatory cell function in patients with active systemic lupus erythematosus. J Immunol 2007; 178:2579–2588.  Back to cited text no. 4
    
5.
Wang X, Wang W, Xu J, Wu S, Le Q, Parizot C. All-trans retinoid acid promotes allogeneic corneal graft survival in mice by regulating Treg-Th17 balance in the presence of TGF-β. BMC Immunol 2015; 16:17.  Back to cited text no. 5
    
6.
Hochberg MC, for the Diagnostic and Therapeutic Criteria Committee of the American College of Rheumatology. Updating the American College of Rheumatology revised criteria for the classification of systemic lupus erythematosus [letter]. Arthritis Rheum 1997; 1725:40.  Back to cited text no. 6
    
7.
Bombardier C, Gladman DD, Urowitz MB, Caron D, Chang DH, Mahadevan S and the Committee on Prognosis Studies in SLE. Derivation of the SLEDAI: a disease activity index for lupus patients. Arthritis Rheum 1992; 35:630–640.  Back to cited text no. 7
    
8.
Crichton N, Wewers ME, Lowe NK, Liang S, Li J, Napierata L. A critical review of visual Analogue scales in the measurement of clinical phenomena. Black well Science Ltd. J Clin Nurs 2001 10:697–706.  Back to cited text no. 8
    
9.
Tang G. Techniques for measuring vitamin A activity from β-carotene. Am J Clin Nutr 2012; 96:1185–1188.  Back to cited text no. 9
    
10.
Furr HC, Green MH, Haskell M, Mokhtar N, Nestel P, Newton S et al. Stable isotope dilution techniques for assessing vitamin A status and bio efficacy of provitamin A carotenoids in humans. Public Health Nutri 2005; 8:596–607.  Back to cited text no. 10
    
11.
Morton RF, Hebel JR, McCarter RJ. [electronic resource], A study guide to epidemiology and biostatistics. 5th ed. Rockville: Md Aspen Publication; 2001. pp. 71–74.  Back to cited text no. 11
    
12.
Pan X, Yuan X, Zheng Y, Wang W, Shan J, Lin F et al. Increased CD45RA + FoxP3low regulatory T cells with impaired suppressive function in patients with systemic lupus erythematosus. PLoS One 2012; 7:e34662.  Back to cited text no. 12
    
13.
Kida Y, Xia Z, Zheng S, Mordwinkin NM, Louie SG, Zheng SG et al. Interleukin-1 as an injury signal mobilizes retinyl esters in hepatic stellate Cells through down regulation of lecithin retinol acyltransferase. PLoS One 2011; 6:e26644.  Back to cited text no. 13
    
14.
D’Ambrosio DN, Clugston RD, Blaner WS, Tao X, Cai L, Wang J. Vitamin A metabolism: an update. Nutrients 2011; 3:63–103.  Back to cited text no. 14
    
15.
Hanly JG, Thompson K, McCurdy G, Fougere L, Theriault C, Wilton K. Measurement of autoantibodies using multiplex methodology in patients with systemic lupus erythematosus. J Immunol Methods 2010; 352:147–152.  Back to cited text no. 15
    
16.
Elias K, Laurence A, Davidson TS, Stephens G, Kanno Y, Shevach EM et al. Retinoic acid inhibits Th17 polarization and enhances FoxP3 expression through a Stat-3/Stat-5 independent signaling pathway. Blood 2008; 111:1013–1020.  Back to cited text no. 16
    
17.
Nolting J, Daniel C, Reuter S, Steulten C, Li P, Sucov H et al. Retinoic acid can enhance conversion of naive into regulatory T cells independently of secreted cytokines. J Exp Med 2009; 206:2131–2139.  Back to cited text no. 17
    
18.
Sobel ES, Brusko TM, Butfiloski EJ, Hou W, Li S, Cuda CM et al. Defective response of CD4+ T cells to retinoic acid and TGF-β in systemic lupus erythematosus. Arthritis Res Ther 2011; 13:R106.  Back to cited text no. 18
    
19.
Bennet RT, Mazzaccaro RJ, Chopta N, Melman A, Franco I, Soylu A et al. Suppression of renal inflammation with vitamins A in lupus nephritis in SLE patients. J Urol 1999; 161:1681–1684.  Back to cited text no. 19
    
20.
Yang J, Yang X, Zou H, Chu Y, Li M, Zou H. Recovery of the immune balance between Th17 and regulatory T cells as a treatment for systemic lupus erythematosus. Rheumatology 2011; 50:1366–1372.  Back to cited text no. 20
    


    Figures

  [Figure 1], [Figure 2], [Figure 3]
 
 
    Tables

  [Table 1], [Table 2], [Table 3], [Table 4]



 

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