Longitudinal Antibody Dynamics Against Structural Proteins of SARS-CoV-2 in Three COVID-19 Patients Shows Concurrent Development of IgA, IgM, and IgG.

BACKGROUND: Dynamics and persistence of neutralizing and non-neutralizing antibodies can give us the knowledge required for serodiagnosis, disease management, and successful vaccine design and development. The disappearance of antibodies, absence of humoral immunity activation, and sporadic reinfection cases emphasize the importance of longitudinal antibody dynamics against variable structural antigens.
METHODS: In this study, twenty-five healthy subjects working in a SARS-COV-2 serodiagnostic assay development project were enrolled, and their sign and symptoms were followed up to six months. Three subjects showed COVID-19-like symptoms, and three subjects' antibody dynamics were followed over 120 days by analyzing 516 samples. We have developed 12 different types of in-house ELISAs to observe the kinetics of IgG, IgM, and IgA against four SARS-CoV-2 proteins, namely nucleocapsid, RBD, S1, and whole spike (S1+S2). For the development of these assays, 30-104 pre-pandemic samples were taken as negative controls and 83 RT-qPCR positive samples as positive ones.
RESULTS: All three subjects presented COVID-19-like symptoms twice, with mild symptoms in the first episode were severe in the second, and RT-qPCR confirmed the latter. The initial episode did not culminate with any significant antibody development, while a multifold increase in IgG antibodies characterized the second episode. Interestingly, IgG antibody development concurrent with IgM and IgA and persisted, whereas the latter two weans off rather quickly if appeared.
CONCLUSION: Antibody kinetics observed in this study can provide a pathway to the successful development of sero-diagnostics and epidemiologists to predict the fate of vaccination currently in place.

Introduction

Worldwide spreading of SARS-CoV-2 caused by the novel coronavirus has a high infectious rate and has already claimed more than 3.5 million deaths till 30 May 2021.1 The previous two severe coronavirus infections in humans, ie, SARS-CoV and MERS-CoV, were epidemic in nature and geographically isolated.2,3

Symptoms associated with prevailing coronavirus infections that cause seasonal colds in humans include sore throat, cough, feverishness, congestion, wheezing, sputum, hoarseness, chills, dyspnea, diarrhea, rhinorrhea, sleep disturbance, muscle pain, fatigue, and joint pain.4–7 Similar to other ordinary human coronavirus infections, SARS-CoV-2 cases can be asymptomatic or symptomatic.8 COVID-19 symptomatic cases show symptoms similar to but often more severe than those presented by other common human coronaviruses. Additional symptoms include ageusia and anosmia, blood pressure fluctuation, myalgia, and severe respiratory complications.9,10 In extreme cases, patients may experience septic shock, metabolic acidosis, coagulation dysfunction, bleeding, organ failures, and even death.11,12

SARS-CoV-2 employs multiple tactics that enhance its prevalence rate. Escape mutation by the virus reduces the immunoglobulin-binding capacity, which can render certain vaccines less effective by reducing the efficacy of neutralizing antibodies, resulting in reinfection.13–17 Additionally, its virulence is enhanced by anchoring non-structural proteins (nsp) in double-membrane vesicles and capping mRNA, respectively, increasing its persistence capability and protecting the genome from intracellular viral host innate immune response.18–22 More than 4000 mutations have been reported for SARS-CoV-2, and the recent variants reported in the UK show cluster mutations in spike with escape mutation from South African variants, challenging long-term efficacies of spike-based vaccines.14,15,23,24

Patients generally develop antibody and memory T-helper cells against that particular virus, there has been a report of the decline of those cells along with Treg cells in severe cases of Covid-19.25,26 Additionally, observations of quick disappearances of neutralizing antibodies and activation of T-cell mediated immunity to eliminate SARS-CoV-2 without involving B-cell mediated immunity in multiple cases have also been reported.27,28 In line with these observations, reinfection/relapse with SARS-CoV-2 has been invoked to explain the recurring presence of SARS-CoV-2 RNA after testing negative by RT-qPCR, a gold standard test for COVID-19 diagnosis.29,30

Recently there has been a few reports of reinfection, there is still a raging debate on its overall frequency of occurrence.14,16,31–43 This raises questions about the efficacy of an effective vaccine. Understanding the behavioral pattern of antibody dynamics against SARS-CoV-2 antigens in a longitudinal study can shine some light on the veracity, or otherwise, of reinfection. Moreover, the success of serodiagnostic relies on proper antibody dynamic studies against proteins under consideration.

This article analyzed the kinetics of antibodies against four structural proteins of SARS-CoV-2 in three RT-qPCR positive patients. Our four monthly observations started 60 days before being RT-qPCR positive, during which time they could have been exposed to coronaviruses and showed coronavirus disease-like symptoms.

Method and Materials

Case History and Clinical Characteristics

A cohort comprising twenty-five people, 15 male, and ten female, was selected for the study. The emergence of COVID-19 in China and its designation as a pandemic in 2020, this team started developing diagnostic kits for SARS-CoV-2 from March 2020 onwards. The subjects were regularly checked for any signs and symptoms, and were under serosurveillance to ensure the quality of the working environment. Among study subjects the three male who were actively involved in developing coronavirus diagnostics and frequently examined for suspected and confirmed COVID-19 through blood and nasopharyngeal, samples, showed COVID-19 like symptoms, were selected for the study. The studied subjects were healthy with no history of chronic disease or administration of any immunosuppressive drugs. Apart from direct exposure to infectious samples, Subject 01 (S01) was enrolled because he had exposure to the 2003 SARS-CoV outbreak and had an accidental exposure to SARS-CoV-2 positive serum parenterally, during inactivation of patient serum at the beginning of May. This led to the development of mild fibrosis around the inoculation site. Subject 02 (S02) and Subject 03 (S03) presented symptoms associated with coronavirus infection at the end of May 2020. This includes high- and low-grade fever, diarrhea, asthenia, sore throat, shortness of breath, and dry cough (). Amid the ongoing pandemic, S02 and S03 took unproven treatment regimens, including ivermectin, doxycycline, paracetamol, normal saline, and vitamin-C and zinc.

Between Mid-June to the first week of July 2020, none of the subjects showed any symptoms associated with COVID-19 except for S02, who experienced sporadic rash and allergic reactions. However, after about 50 days from first exposure or symptoms, all three presented COVID-19-like symptoms, such as high-grade fever, blood pressure fluctuation, ageusia, anosmia, nausea, severe weakness, confusion, and muscle pain followed by sore throat, dry cough, slight respiratory distress, diarrhea, insomnia, and increase in urination (). They tested positive for COVID-19 by RT-qPCR at the end of July.

Reverse Transcriptase Quantitative Real-Time PCR

RT-qPCR was done using patients’ oropharyngeal swabs. Two SARS-CoV-2 specific genes (N1 and N2) for the conserved nucleocapsid (N) protein region were targeted and simultaneously amplified. For total RNA extraction QIAamp Viral RNA Mini Kit was used, and purity of RNA was confirmed spectrophotometrically (Thermo Scientific, NanoDrop 2000c). From total RNA RT-qPCR was carried out using QIAGEN OneStep RT-PCR Kit with CDC 2019-nCoV Real-Time RT-PCR Diagnostic Panel.

Blood Sample Preparation to Investigate Antibody Dynamics

The patient’s blood was collected at various time intervals before the primary infection until 120 days. Blood was collected by venipuncture in tubes containing clotting factors. Later, serum was separated by centrifugation at 3500 rpm for 15 minutes at room temperature. The serum samples were stored at −80°C until further investigation. For negative control, two years old 30–104 serum samples from healthy subjects were applied. Moreover, as the positive control, 83 COVID-19 RT-qPCR positive serum samples were used.

Antibody Dynamics Analysis by in-House ELISA

The antibody profile of subjects was determined using in-house ELISA. We primarily investigated both the neutralizing (anti-receptor binding domain (RBD-IgG) and anti-Spike (S1-IgG) and non-neutralizing antibodies (anti-N-IgG) in patients’ serum using our in-house ELISA method.44,45 Briefly, commercially obtained RBD, S1, and N proteins (Sino Biological, China) were coated on ELISA plates (ExtraGene, USA). After blocking, diluted (1:100) serum samples were applied, and SARS-CoV-2 specific human IgG, IgM, and IgA were detected using HRP tagged goat anti-human IgG (The Native Antigen, UK), goat anti-human IgM (Abcam, USA), and goat anti-human polyclonal IgA (Sigma-Aldrich, USA). Furthermore, we investigated antibody dynamics against S1+S2 (Sino Biological, China) using the similar method. Results were obtained by a microplate reader (Thermo Scientific, USA) at 450 nm.

Statistical Methods

Data were presented as either mean, median, and standard deviation. Spearman rank correlation was used to evaluate the bivariate association between different in-house ELISA techniques. An independent sample t-test was used to see the difference in fold change of OD/cut-off value between the first and second episodes of infection. Paired sample t-test was used to see the change in OD/cut-off values of antibodies between the participants. All analyses were performed with Stata 13 (StataCorp, LP, College Station, Texas, USA). The graphical presentation was made using GraphPad Prism 8.3 or MS. Excel. A p-value <0.05 was considered significant.

Results

Twelve different types of ELISA were developed for this study, where IgA, IgM, and IgG antibody fold increased were measured against SARS-CoV-2 N, RBD, S1, and S1+S2 proteins. The sensitivity and specificity of each ELISA were measured separately (–), and ROC curves were prepared for OD to Cut-off ratio for 0.95 and 1.0 for each assay (–).

Antibodies developed in the three test subjects were measured using an in-house ELISA against SARS-CoV-2 specific antigens, ie, N, S1, whole spike (S1+S2 ECD), and RBD. Serum samples were taken at 14, 16, and 13-time points from S01, S02, and S03, respectively, over four months while observing the dynamics of IgA, IgM, and IgG antibodies against four SARS-CoV-2 specific proteins mentioned above. Graphs were plotted, and correlations were assessed using a total number of 516 observations (Figures 1–3; ; –).

All three subjects showed mild elevation of IgG against N protein in their first episode, which continued to persist till the second episode (Figure 1). In the second episode, the sharp rise of these antibodies was observed, which continued to persist at a 7–12-fold increase compared to the first episode (p<0.001) for about 60 days till the end of our study (Figures 1 and 2). Initial elevation can confer cross-reaction against other coronaviruses, as observed for S01 (Figure 1).46 It is to be noted that the subjects did not undergo SARS-CoV-2 RT-qPCR during the first episode, though they did manifest antibody levels higher than two years old negative samples.

Figure 1

Antibody dynamic of IgA, IgM, and IgG of the three subjects (S01, S02, S03) against SARS-CoV-2 nucleocapsid (N), receptor-binding domain (RBD), N-terminal of spike protein (S1), and spike protein (S1+S2) (A–L). Figure (A, E and I) represents antibody dynamics against nucleocapsid; (B, G, and J) against RBD; (C, G, and K) against S1; whereas (D, H, and L) against S1+S2 in S01, S02, and S03, respectively. IgG’s increase was consistent in all three subjects though there were some dissimilarities in the IgM and IgA antibody titer among them. However, the second exposure led to a multifold increase of IgG against all four SARS-CoV-2 proteins. In contrast, S01 failed to elicit an increase in IgA against SARS-CoV-2 proteins except for a four-fold increase against whole spike protein. Similarly, S03 failed to elicit IgM response against all four antigens.

Figure 2

Antibody expression during symptomatic episode 1 and symptomatic episode 2. IgG expression during symptomatic episode 2 was higher when compared to symptomatic episode 1 in all the subjects studied. The higher levels of antibodies correlate with the severity of the symptoms of the subjects.

IgM dynamics against N, on the other hand, was variable, where S01 had a higher IgM fold compared to S02 (p<0.001) and S03 (p=0.001), while both S02 and S03 showed no significant difference (data not shown). The subject S03 continued to show a persisted elevation of 1.65-fold anti-N IgA throughout the study (Figure 1). Interestingly, when N-IgA, N-IgM, and N-IgG in all three subjects were compared with RBD antibodies against the respective class, N-IgG showed the highest correlation with RBD-IgG (rs=0.902; p<0.001) (Figure 3). Although, in the individual level, S01 and S03 showed insignificant correlation for IgA, rs=0.262; p=0.336 and rs=0.369; p=0.215, respectively ().

Figure 3

Correlation of the anti-RBD antibody compared with anti-NCP, anti-S1, and anti-S1+S2 in S01, S02, and S03. In all the subjects, the increase in anti-RBD correlated with the increase in anti-S1. The first episode in all the graphs is signified with the cluster formed at the lower end of the x- and y-axis.

Concerning RBD and S1, none of the participants presented any increase in the first episode (Figure 1). In contrast, the second episode statistically significantly increased (p<0.001) almost 11-fold (first episode: 1.29±0.42; second episode: 13.80±5.00) in IgG against RBD (Figure 2). Similarly, an almost eightfold increase (first episode: 1.32±0.23; second episode: 10.05±5.42) in IgG against S1 (p<0.001) was also evident (Figure 2). The antibody was dynamic of RBD and S1 highly correlated (rs=0.923; p<0.001) (Figure 3). In all three subjects, after the sharp rise in IgG against RBD and S1 (8–20-fold), it plateaued to a 7–10-fold increase during the two months observation (Figure 1).

Like that of correlation between S1-IgG in all three subjects, S1-IgM also correlated significantly, rs= 0.898; p<0.001, with their respective RBD antibodies (Figure-3). Although anti-RBD and anti-S1 IgM titers in the three subjects varied at the individual level (Figure 1). While S01 and S02 presented more than a threefold increase, such increase was absent in S03 (Figure 1). Similar trend was observed for anti-N IgM (rs= 0.393; p=0.164) in S01 (Figure 1; ) and anti-S1 IgM (rs= 0.632; p=0.021) for S03, compared to their respective RBD antibodies (Figure 1; ).

However, in contrast to IgM and IgG, S02 presented the highest anti-RBD IgA (22.5-fold) and anti-S1 IgA (17.8-fold) increase compared to S01 (6.1-fold, 9.4-fold, respectively) and S03 (5.8-fold, fourfold, respectively) (Figure 1). Moreover, overall anti-S1 IgA (rs= 0.872; p<0.001) increase was comparable to anti-RBD (Figure 1; Figure 3). Although, anti-S1 IgA dynamics of S02 and S03 correlate highly, rs= 0.875; p<0.001 and rs= 0.927; p<0.001, respectively, compared to their RBD-IgA (Figure 1; ), S01 did not present any increase in IgA for either of the SARS-CoV-2 proteins (Figure 1).

Whole spike proteins (S1+S2) have the propensity of expressing domains that may cross-react with other coronaviruses (Figure 1).46,47 In subject S01, the trend of IgM and IgA antibody dynamics against anti-whole spike closely mimics that of anti-N protein (Figure 1; and ). There was an approximately 3.5 and 4-fold increase of anti-whole spike IgM and IgA, respectively, in the second episode. Additionally, anti-whole spike IgG increased significantly (p<0.001) in the second episode (5.70±1.89) when compared with the first episode (2.71±1.40) (Figure 2). The IgM against whole spike proteins persisted for two weeks for subjects S01 and S02 but never increased for S03 (Figure 1). Surprisingly, all three subjects showed abrupt IgA rise against this protein when IgG started to wade off (Figure 1).

Discussion

Our study looks into antibody dynamics of COVID-19 and how they correlate with the disease outcome with symptoms. Fortunately, all three subjects survived the infection but with varying degrees of post-COVID-19 effects. In all three subjects, the first episode of symptoms cannot be conclusively defined as SARS-CoV-2 infection due to the lack of RT-qPCR testing results. However, the subjects presented a pool of symptoms that are common for coronavirus infection, indicating the possibility of being infected with SARS-CoV-2 or with other species of coronavirus.4

Upon investigating antibody dynamics, it was observed that in the first episode, all the subjects presented a slight rise in anti-N and anti-whole spike protein (S1+S2), while such development being absent for anti-RBD and anti-S1 antibodies. Both S02 and S03 peaked for the antibodies mentioned above after 20 days of symptom onset in the second phase. We suspect the first episode may have been due to infection with any of the common coronaviruses. This is mainly due to approximately 24.6–90.5% similarity of the nucleocapsid sequences shared amongst the coronaviruses.48 Furthermore, it has also been noted that the S2 region is conserved within members of the Coronaviridae family members while the S1 region varies.49,50 Henceforth, there is a possibility of infection with any other common coronaviruses (Figure 4).

Figure 4

Probable causes for two episodes of symptoms. The first episode did not present a significant antibody increase. The symptoms presentation during the first episode may be due to cross-reacting coronavirus infection. Medication may have resulted in the suppression of antibody development during the first episode. In addition to it, lack of Th2 cell-mediated immunity activation in the first episode may cause the lack of antibody development. This, in turn, may lead to virus persistence or viral reinfection, resulting in a second episode of the presentation of the symptoms, which may have led to activation of Th2 cell-mediated immunity.

Another observation is that for S01, the anti-N and anti-(S1+S2) increase was maintained continuously until the second episode. This anomaly may be explained due to S01’s previous exposure to SARS-CoV during the 2003 outbreak. The exposure may have played a significant role in maintaining the antibody titer of anti-N and anti-(S1+S2), while S02 and S03 presented a sharp decline. Nevertheless, previous exposure did not cross-protect against SARS-CoV-2, as S01 suffered from symptomatic COVID-19 symptoms like others while the neutralizing antibodies formed 10–12 days after symptom onset (Figure 4).

The second episode is characterized by the sharp increase in antibody titer (Figures 1–3). The multi-fold rise in the antibody titer was observed approximately 12 days from the onset of symptoms mentioned in earlier reports.51,52 However, during the study period, the subjects did not lose the antibody titer, ultimately contributing to their immunity from subsequent infection with SARS-CoV-2. However, they all experienced from post-COVID-19 and again COVID-19-like symptoms, nevertheless, were repeatedly revealed negative for SARS-CoV-2 RNA at RT-qPCR tests. The antibody titer’s dynamic increases against the four viral proteins highly correlated with the symptoms’ severity in all subjects. Though an increase in IgG was consistent throughout the subjects, there was some dissimilarity in the IgM and IgA antibody titer.

IgA antibody protects from viruses by blocking its binding onto the mucosal membrane.53,54 Previous studies mention the development of IgA before the development of IgM.55 There also have been reports that the early development of IgA would provide better protection by neutralizing the viruses at the site of infection.53 Our study presented IgA antibodies’ development against the four proteins for S02, which coincide with the subject’s symptoms with epithelial lining, like severe diarrhea, although no respiratory involvement was observed. In the case of S01 and S03, IgA increased multifold against whole-spike protein only.

Similarly, IgM development before IgG or vice versa may decide the outcome and severity of the disease.51 In S01, IgM development was absent during both the first and second episodes, which the previous exposure hypothesis can explain. Furthermore, the subject did recover early after a short bout of the severity of symptoms. In previous reports, the development of IgG before the development of IgM signified less severity of the symptoms in subjects.51 One interesting observation in our study was for both the S01 and S02, and there was an increase in IgM for whole-spike protein but not for RBD and S1 proteins in the second episode. This would signify that the IgM increase was for the S2 part of the whole spike protein rather than the S1 part. Our observation coincides with SARS-CoV’s previous findings where IgG developed simultaneously with IgM and IgA.56 Moreover, IgM and IgA disappeared rapidly in all three cases, indicating a unique class-switching phenomenon, which needs to be confirmed with a large population study.

At the end of the study, the IgG antibody titers against all SARS-CoV-2 proteins, essentially N, RBD, and spike, remained high. However, further, observation is required to identify the overall titer of antibodies over two to three years. It is noted that SARS-CoV and MERS-CoV are known to protect for 2–3 years approximately.57,58

One of our study’s main limitations is that it presents only three subjects and the same gender. The lack of diversity may result in the skewness of our conclusion. However, though our study is limited to three subjects, the significance lies in the difference of antibody development in different individuals due to underlying various physiological conditions. Additionally, it also provides direct evidence of the correlation between the severity of disease and antibody development.59 This information would provide the researchers with a starting point to study antibody development dynamics after vaccination. It would also provide insights into the persistence of antibodies after being exposed to the SARS-CoV-2 virus. Moreover, our study would help researchers design effective IgM/IgG/IgA serodiagnostic kits by selecting the SARS-CoV-2 specific proteins.

Recommendations

On the event of SARS-CoV-2 infection, it is essential to observe the antibody levels.

The early presentation of IgG or IgM would provide a better idea about the probability of the severity of the infection.

Further investigation is to be carried out to observe the correlation of IgA with the outcome of the infection.

Antibody levels are to be observed after vaccination with SARS-CoV-2.

Observation of antibody levels is necessary to analyze the probability of reinfection with SARS-CoV-2.

Further studies with larger sample size and more extended periods are required to establish the facts provided in this study.