Use of a Chagas Urine Nanoparticle Test (Chunap) to Correlate with Parasitemia Levels in T. cruzi/HIV Co-infected Patients

 

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Abstract

Fig 1

Antigenic bands in nanoparticles-concentrated urine samples of patients with HIV/T. cruzi co-infection.

Bands were detected by Western Blot using a monoclonal antibody anti-lipophosphoglycan of T. cruzi. Bands of 20 kDa, 42 kDa, 58 kDa, 75 kDa, 82 kDa were considered specific for T. cruzi. Bands of other molecular weight were not considered for diagnosis criteria. Urine samples of T. cruzi+/HIV+ patients: Lanes 1–3, 5, 7, 9, 10–11, 13–14. Urine samples of T. cruzi-/HIV+ patients: Lanes 4, 6, 8, 12, and 15.

Table 2

Percentages of positive patients detected by Chunap stratified by levels of parasitemia among HIV/T. cruzi infected patients.

	Chunap	Micromethod	qPCR	Serology
Reactivation or high parasitemia (n = 7)	7 (100%)	7 (100%)	7 (100%)	7 (100%)
Moderate parasitemia (n = 12)	11 (91.7%)	0 (0%)	12 (100%)	12 (100%)
Negative parasitemia (n = 12)	5 (41.7%)	0 (0%)	0 (0%)	12 (100%)

Confirmation of T. cruzi infection was based on positive results by 2 or more of serological tests for detection of anti-T. cruzi IgG.

Chunap and correlation with levels of parasitemia

Mean levels of parasitemia were significantly different between patients with reactivation of Chagas disease (3.28 logarithm copy number of parasites/ml, 95% CI: 1.56 to 5.00) and patients without reactivation but with positive qPCR (1.43 logarithm copy number of parasites/ml, 95% CI: 1.13 to 1.72) (p = 0.003) (Table 3) (Fig 2A). Similarly, mean levels of antigenuria were significantly higher in patients with high parasitemia or reactivation of Chagas disease (mean = 242.21pg, 95% CI: 125.45 to 358.95) compared to patients with moderate parasitemia (mean = 43.32 pg, 95% CI: 25.06 to 61.58) (p<0.001) (Fig 2B). Using 105 pg as a cut-off, Chunap could detect all patients with reactivation (7/7). The best balance between specificity (90.62%, 3/29) and sensitivity (71.43%, 5/7) for determination of reactivation by qPCR was obtained with the cut-off of 2 log (parasites/ml blood), this cut-off was used for categorization of parasitemia levels in the regression model. High variability of parasitemia levels measured by qPCR was observed, even in a logarithmic scale.

Table 3

Linear regression model for prediction of levels of antigenuria by levels of parasitemia, and relationship with immune status, HIV load, sex, age and initiation of antiretroviral therapy.

	Unadjusted			Adjusted
	Coefficient	95% CI	p-value	Coefficient	95% CI	p-value
Log parasitemiaa
< 2.0	31.52	17.04 to 46.01	<0.001	33.65	17.48 to 49.82	<0.001
≥ 2.0	106.00	85.13 to 126.85	<0.001	101.42	79.98 to 122.86	<0.001
CD4 classificationb
>500 cells	Reference			Reference
200–500 cells	-27.63	-94.80 to 39.54	0.412	-0.30	7.28 to 64.88	0.983
< 200 cells	22.37	-45.56 to 90.28	0.511	36.08	7.28 to 64.88	0.016
CD8 classificationc
> 1000 cells	Reference			Reference
500–1000 cells	-4.29	-69.39 to 60.81	0.895	7.71	-20.97 to 36.39	0.550
<500 cells	-1.72	-70.67 to 67.23	0.960	12.40	-17.58 to -42.38	0.407
HIV loadd
>30 000	Reference			Reference
5000–30 000	-49.83	-107.64 to 7.98	0.089	18.72	-10.06 to 47.50	0.195
< 5000	2.42	-87.47 to 92.31	0.957	36.85	-4.70 to 78.40	0.080
Age (years)	-0.27	-2.20 to 1.66	0.782	-1.23	-2.06 to -0.40	0.005
Sex (male versus female)	56.25	5.07 to 107.42	0.032	23.67	-0.87 to 48.21	0.058
ART (yes versus no)	-48.43	-100.41 to 3.56	0.067	-0.11	-23.87 to 23.64	0.992

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^a Logarithm of copy number of parasites/ml blood.

^{b, c} cells/ml of blood,

^d Copy number of HIV virus/ml blood.

ART: Antiretroviral treatment.

 

Fig 2

Levels of parasitemia and antigenuria in T. cruzi/HIV co-infected patients.

A.) Levels of parasitemia determined by qPCR in T. cruzi/HIV co-infected patients. B.) Levels of antigenuria determined by Chunap in the three groups of T. cruzi/HIV co-infected patients. Levels of parasitemia: High parasitemia = positive by PCR and microscopy, Moderate parasitemia = positive by PCR, and negative by microscopy, Negative parasitemia = negative by PCR and microscopy but positive by serology, and No Chagas = negative by microscopy, PCR and serology. Bottom and top limits of the boxes correspond to first and third quartiles, and the line inside the boxes represents the second quartile (median). P-values were calculated using T-test with equal variances. * Statistically significant difference.

A linear relationship was observed between antigenuria and parasitemia levels in both the unadjusted and adjusted regression model (Table 3). Interestingly, when levels of parasitemia were less than two logarithms, the expected increase in levels of antigenuria was 31.52 pg (95% CI: 17.04 to 46.01) per each increase in one logarithm of parasitemia (p<0.001, adjusted r² = 0.84) (Table 3). Similarly, when levels of parasitemia were higher than two logarithms, the expected increase in antigenuria levels was 106.00 pg (95% CI: 85.13 to 126.85) per each increase in one logarithm of parasitemia (p<0.001, adjusted r² = 0.84) (Table 3).

Chunap, host factors and HIV infection

Among patients with Chagas disease, mean levels of CD4+ T-cell counts were significantly lower in patients with reactivation (131 cells, 95% CI: -56.54–318.54) compared to patients without reactivation (322.46 cells, 95% CI: 229.45–415.47) (t-test with unequal variances: p = 0.046) (Fig 3A). Clinical manifestations, parasitemia levels and immunosuppression status of each patient are shown in Table 4. Among patients with reactivation of Chagas disease, 3 showed clinical manifestations related with Chagas neurological disease, 1 patient had an intestinal perforation, and 3 patients did not show any clinical manifestations. An increase in levels of antigenuria of 36.08 pg (95% CI: 7.28 to 64.88, p = 0.016) in patients with < 200 CD4+ T-cell counts was observed in the adjusted linear regression model as compared to patients with >500 CD4+ T-cell counts (Table 3), but no differences were observed in the unadjusted model. No statistical associations were observed between antigenuria levels and CD+8 cells counts, HIV load, and ART in the regression model. There was a trend to lower mean levels of CD8+ T-cell counts between the two groups (reactivation group = 429.6 cells, Non-reactivation groups = 838.42 cells, t-test with unequal variances: p = 0.064) (Fig 3B). HIV viral loads were not statistically significantly different between patients with reactivation (mean: 134,303 copies/ml, 95% CI: -35,516 to 304,122) and without reactivation (mean: 121,761 copies/ml, 95% CI: -62,834 to 306,355) (Student’s t-test with unequal variances: p = 0.901).

 

 

Fig 3

Counts of T-cell CD4+ and T-cell CD8+ in T. cruzi /HIV co-infected patients.

(A) T-cell CD4+ and (B) T-cell CD8+ cells. Bottom and top limits of the boxes correspond to first and third quartiles, and the line inside the boxes represents the second quartile (median). P-values were calculated using T-test with unequal variances. * Statistically significant difference.

Table 4

Clinical characteristics, antigenuria and parasitemia levels and immunosuppression status of HIV/T. cruzi co-infected patients.

Reactivation cases: detectable parasitemia by microscopy
CODE	T-cell CD4+a	T-cell CD8+b	HIV loadc	Chunapd	Parasite loade	Clinical manifestationsf	ARTg	Died
1	179	624	83653	432.1	5.6	Transverse myelitis	No	Yes
2	ND	ND	ND	396.7	5.4	CNS mass lesions	No	Yes
3	3	78	237684	255	3.5	None	Yes	No
4	ND	ND	ND	108.5	3.4	None	No	No
5	373	533	15301	142.9	2.9	None	No	No
6	71	852	17088	172.3	1.1	Meningitis	No	Yes
7	29	61	317789	188	0.9	Intestinal perforation	Yes	Yes
Mean	131	429.6	134303	242.2	3.3
SD	151	348.7	136767.1	126.3	1.9
Moderate parasitemia: undetectable parasitemia by microscopy but qPCR positives
CODE	T-cell CD4+a	T-cell CD8+b	HIV loadc	Chunapd	Parasite loade	Clinical manifestationsf	ARTg	Died
8	231	1033	120282	89.9	3.2	None	No	No
9	48	426	652536	22.7	2.2	None	No	No
10	497	ND	ND	54.3	2.1	None	Yes	No
11	ND	ND	ND	52.4	1.9	None	No	No
12	132	1615	69402	58.3	1.9	None	Yes	No
13	659	1527	ND	47.2	1.5	None	No	No
14	303	1093	7711	19.6	1.4	None	No	No
15	265	1336	68	42.7	1.4	None	Yes	No
16	328	898	40	99.9	1.3	None	Yes	No
17	532	1052	2706	24.9	1.2	None	No	No
18	168	417	121339	51.3	0.9	None	No	No
19	383	1052	ND	0	0.9	None	Yes	No
Mean	322.4	1044.9	121760.5	46.9	1.7
SD	184.1	400.5	220801.3	32.2	0.6
Negative parasitemia: undetectable parasitemia by microscopy and qPCR
CODE	T-cell CD4+a	T-cell CD8+b	HIV loadc	Chunapd	Parasite loade	Clinical manifestationsf	ARTg	Died
20	125	224	169815	22.3	0	Alterations in EKG	Yes	No
21	529	778	40	18.4	0	None	Yes	No
22	848	2000	3235	0	0	None	No	No
23	99	1352	1	0	0	None	Yes	No
24	562	ND	ND	0	0	None	Yes	No
25	68	1235	53	27.8	0	Alterations in EKG	Yes	No
26	563	ND	1576	0	0	None	Yes	No
27	105	491	3001633	0	0	None	Yes	No
28	210	562	39227	0	0	None	Yes	No
29	287	1579	ND	0	0	None	Yes	No
30	143	589	150	21.5	0	None	Yes	No
31	108	425	ND	32.3	0	None	Yes	Yes
Mean	303.9	923.5	357303.3	24.5
SD	256.4	582.9	993176.6	5.5

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^{a, b} cells/ml of blood.

^c copy number of HIV virus/ml blood.

^d pg of T.cruzi antigens.

^e Copy number of parasites/ml blood.

^f Clinical manifestations related to Chagas disease.

^g Antiretroviral treatment.

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Discussion

Reactivation of Chagas disease in HIV patients is a serious medical condition, which is often life-threatening. Early diagnosis of Chagas reactivation and prompt treatment can be life-saving. However, current methods are based on microscopy that have sub-optimal sensitivity that do not detect reactivation until parasite loads are very high. A sensitive, non-invasive test is needed to monitor increase in parasitemia levels and predict risk of reactivation. In this study we introduce the potential use of a nanoparticle-based tool to monitor T. cruzi infection in urine of HIV patients.

Chagas and HIV infection

No differences were observed in HIV loads, CD4+ cell and CD8+ cell count, and presence of other co-infections between HIV patients with and without Chagas disease. Among patients with positive serology for Chagas disease, patients with reactivation of Chagas disease had low levels of CD4+ T-cells counts compared to patients without reactivation, as previously observed [15]. The percentage of mortality attributed to Chagas disease was 16.12% (5/31), which is similar to the reported in longitudinal studies (15.09%, 8/53) [10].

Clinical manifestations related to Chagas disease were observed in the nervous system [7, 10]. In the case of the patient with intestinal perforation we were not able to perform a biopsy analysis to make the confirmatory diagnosis; however, intestinal perforation is a complication described in patients with digestive system abnormalities associated with Chagas disease [36]. The presence of asymptomatic reactivation has been previously described and is thought to be an early stage of Chagas reactivation and a risk factor of HIV progression [10, 37].

Performance of Chunap in the diagnosis of Chagas disease

An IgM monoclonal antibody against T. cruzi lipophosphoglycan (LPG) was used in this study for antigen detection. The T. cruzi LPG is a surface glycoconjugate which is composed mainly of glucosamine, sialic acid and galactosamine in the carbohydrate portion, and of alkylacylphosphatidylinositol in the lipid portion [38]. Although this antigen has been primarily characterized in the epimastigote form, it could be an important component of the trypomastigote form, and could be used during cell recognition, invasion, and immune suppression of the host [38]. This antibody recognizes two bands of 42 kDa and 82 kDa in the trypomastigote secretory-excretory antigen and crude sonicated trypomastigotes [26].

The percentage of antigenuria positives detected by Chunap (74%) among those with positive serology is similar to that reported before in chronic infected patients (60%-84%) [39–40]. Two false positive results were found in urine samples of patients with negative serology; one of whom was also co-infected with M. tuberculosis. We hypothesize that the presence of false positives could be explained by the existence of other co-infections. In the case of tuberculosis, the mycobacterial lipoarabinomannan has been detected in urine samples of HIV co-infected patients [41]. The lipophosphoglycan is also found in other infectious agents such as Leishmania, Trichmonas, and Pneumocystis, but the anti-IgM LPG antibody used in this study does not show cross-reaction with the LPG from Leishmania and Trichomonas species [38]. However, further studies are needed in order to assess cross-reaction with other parasites that are commonly present in HIV, such as Toxoplasma gondii, and bacteria and fungi such as M. tuberculosis and Cryptococcus neoformans.

Chunap and relationship with parasitemia levels

Definition of a parasite load threshold for prediction of reactivation could be used as a guide in the use of anti-trypanosomal therapy. The early increase in parasitemia may not be symptomatic as previously described in one prospective study [10], so monitoring for asymptomatic parasitemia may permit early detection of reactivation. This could lead to accelerating the initiation of anti-trypanosomal therapy, which could prevent irreversible damage or death.

Levels of parasitemia, determined by qPCR, were higher in patients that had reactivated Chagas disease than in those without reactivation. However, there was a high variability of parasitemia levels between individuals. This observation was also reported by a previous study (mean ± SD in reactivation cases VS non-reactivation: 12,584.96 ± 11,368.35 VS 10.43 ± 3.53, respectively) [15]. The high variability in parasitemia levels detected by qPCR could be explained by differences in the strains of T. cruzi, and by the inability to distinguish DNA from living and dying parasites [15]. Although there was a wide SD found among antigenuria levels, the variability was less than that seen in parasitemia. This could be explained due to lipophosphoglycan only being excreted by living parasites [38].

In this study, reactivation was defined as the detection of circulating parasites in blood by microscopy with or without the presence of clinical manifestations [10]. This definition has limitations because of the lack of sensitivity and reproducibility of microscopy. As observed by us and others, patients with positive microscopy could have low levels of parasitemia by qPCR (and vice-versa), suggesting a poor correlation between microscopy and qPCR. For example, in the case of patient number 9 in Table 4, the levels of parasitemia and viremia were high, and the CD4+ counts was low. Yet this patient had undetectable parasitemia by microscopy, thus not meeting the reactivation criteria. A better definition of Chagas reactivation is needed so that immunosuppression status and HIV load are also taken into consideration. This will guide clinicians in case management.

In the guinea pig model of Chagas disease and congenital Chagas disease, the presence of antigens in urine is correlated with high levels of parasitemia [19, 26]. In this study we demonstrate that antigenuria levels are positively related with parasitemia levels in humans. Interestingly, the increase in levels of antigenuria was greater among patients with higher levels of parasitemia (> 2 logarithm copy number parasites/ml). All patients with levels of antigenuria higher than 105 pg were patients that showed reactivation. In this cross-sectional study, we have evaluated patients that have reactivated Chagas disease, a longitudinal study will be necessary to determine a cut-off of antigenuria that predicts reactivation and could be used in low-resource settings where serial evaluations of samples are logistically difficult [15].

Chunap and host factors

Antigenuria levels were significantly higher in patients with < 200 CD4+ T-cells, but only in the adjusted model, suggesting possible confounding effects of HIV loads, treatment, age, and sex. In contrast to a previous study, we could not find statistically significant differences between levels of parasitemia or antigenuria, and HIV load and CD8+ T-cells levels [15]. Limitations of this study include possible confounding effects of HIV treatment and the small sample size. Although we adjusted by the use of ART to make statistical comparisons, we could not account for the duration of ART. ART drugs have a direct and more immediate effect on HIV loads as compared to levels of CD4+ T-cells and CD8+ T-cells [15].

Among patients with Chagas disease, young age was found to be a risk factor for high antigenuria levels in the adjusted model. However, this association could be influenced by the time of diagnosis of HIV infection and ART.

The Chunap reached sensitivity levels comparable to the more expensive and time consuming standard of care micromethod and qPCR. The feasibility data presented herein provide evidence that Chunap is a promising tool to improve current Chagas diagnostic algorithm in clinical settings. Furthermore, in a previous study we demonstrated that Chunap protect T. cruzi antigens from degradation [26].

In future studies, poly(NIPAm/TB) particles will be magnetized in order to simplify the clinical diagnostic process and extend accessibility. Sensitivity can be further improved by increasing the volume of urine analyzed. In conclusion, an antigen urine test for monitoring Chagas reactivation in HIV patients would be highly desirable for these reasons: a) levels of antigens in urine are related to levels of parasitemia b) antigenuria levels are less variable compared to levels of parasitemia c) urine is a preferred, less-infectious, non-invasively collected biological fluid that is more acceptable by patients (especially if continuous samples are needed), and d) antigen testing can be scaled to a rapid, point of care test that can be performed in low-equipped laboratories.

Members of the Chagas/HIV Working Group in Bolivia and Peru

Jean Cabeza, Roni Colanzi, Daniel Lozano, Gonzalo Borda, Gerson Galdos, Lisbeth Ferrufino, Louisa Messenger, Rosmery Gross, Leny Sanchez, Omar Gandarilla, Maurus Dorn, and Helena Jahuira.

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Supporting Information

S1 Fig

Linear regression and 95% CI for densitometric quantification of trypomastigote excretory-secretory antigen (TESA) spiked in normal human urine (concentrations 5 pg, 10 pg, 50 pg, 250 pg, 500 pg) and concentrated and detected using Chunap.

(TIF)

Click here for additional data file.^{(694K, tif)}

S1 Checklist

STARD checklist.

Use of Chunap for detection of Chagas disease in T.cruzi/HIV co-infected patients.

(PDF)

Click here for additional data file.^{(513K, pdf)}

S1 Diagram

STARD diagram.

Use of Chunap for detection of Chagas disease in T.cruzi/HIV co-infected patients. * Confirmation of T. cruzi infection was based on positive results by 2 or more serological tests for detection of anti- T. cruzi IgG antibodies. ** Reactivation of Chagas disease was based on the detection of circulating parasites by microscopy.

(TIF)

Click here for additional data file.^{(985K, tif)}

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Acknowledgments

Heydi Castro Sesquen and Santiago Saldaña for the administrative assistance, and JB PHU and Sara D for technical assistance.

The article was partially presented in the 62nd Annual Meeting of the American Society of Tropical Medicine and Hygiene (ASTMH), November 2013, Washington, D.C. Abstract Number: 1423.

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Funding Statement

This work was supported by the National Institutes of Health [5 R24 TW007988, D43 TW006581, D43TW008273, P50 AI074285, 1R33CA173359-01, and 1R21AR061075-01]. The funder had no role in study design, data collection and analysis, decision to publish, or preparation of the manuscript.

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Data Availability

All relevant data are within the paper.

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