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Academic literature on the topic 'Plasmodium vivax (PV)'
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Journal articles on the topic "Plasmodium vivax (PV)"
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Haspreet, Kaur Gill, Kumari Swarnim, and Jaiswal C.P. "A Hospital Based Assessment of the Diagnostic Efficacy of Two Different Approaches in the Diagnosis of Malaria." International Journal of Current Pharmaceutical Review and Research 16, no. 05 (2024): 644–47. https://doi.org/10.5281/zenodo.12886193.
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AbstractAim: Evaluation of Rapid diagnostic tests compared to peripheral smear in the diagnosis of malaria.Methods and Materials: This is a retrospective hospital-based study was conducted in the Department ofpathology, NMCH, Patna, Bihar, India for 9 months. During this period, 1835 blood samples were received formalaria diagnosis from clinically suspected cases. Blood samples were collected in EDTA vacutainer tube.Peripheral smears were made on a clean glass slide with a drop of blood, air dried and stained with Leishmanstain. Smears were thoroughly examined under oil immersion for the presence of malaria parasite. Of 1835samples, 600 samples were randomly selected and Rapid Diagnostic test was performed using Antigen based Pf(HRP-II) and PV (pLDH) specific kit. Procedure was performed as per manufacturer’s instructions.Results: Of the 600 Peripheral smears studied, 175 showed positive for malarial parasite. Plasmodium Vivax (Pv)was diagnosed in 173 Cases, Plasmodium Falciparum (Pf) was identified in one case and one smear showed mixedinfection with both Plasmodium Vivax and Plasmodium Falciparum. Rapid Diagnostic test showed 189 positivecases, of which 178 were plasmodium Vivax, four cases were Plasmodium Falciparum and seven cases showedmixed infection with Falciparum and Vivax. Sensitivity, specificity, Positive Predictive Value and NegativePredictive value were 100%, 96.7%, 92.5% and 100% respectively.Conclusions: Peripheral smears are considered to be gold standard for diagnosis of malaria. RDTs can be moresensitive and specific than peripheral smears. Newer Pf /Pv specific antigen card can distinguish mixed and PFinfections. However further studies are required to assess cost effectiveness and efficiency of different RDTs.
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Jang, Woong Sik, Da Hye Lim, YoungLan Choe, et al. "Development of a Multiplex Loop-Mediated Isothermal Amplification Assay for Diagnosis of Plasmodium spp., Plasmodium falciparum and Plasmodium vivax." Diagnostics 11, no. 11 (2021): 1950. http://dx.doi.org/10.3390/diagnostics11111950.
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Malaria, caused by the parasite Plasmodium and transmitted by mosquitoes, is an epidemic that mainly occurs in tropical and subtropical regions. As treatments differ across species of malarial parasites, there is a need to develop rapid diagnostic methods to differentiate malarial species. Herein, we developed a multiplex malaria Pan/Pf/Pv/actin beta loop-mediated isothermal amplification (LAMP) to diagnose Plasmodium spp., P. falciparum, and P. vivax, as well as the internal control (IC), within 40 min. The detection limits of the multiplex malaria Pan/Pf/Pv/IC LAMP were 1 × 102, 1 × 102, 1 × 102, and 1 × 103 copies/µL for four vectors, including the 18S rRNA gene (Plasmodium spp.), lactate dehydrogenase gene (P. falciparum), 16S rRNA gene (P. vivax), and human actin beta gene (IC), respectively. The performance of the LAMP assay was compared and evaluated by evaluating 208 clinical samples (118 positive and 90 negative samples) with the commercial RealStar® Malaria S&T PCR Kit 1.0. The developed multiplex malaria Pan/Pf/Pv/IC LAMP assay showed comparable sensitivity (100%) and specificity (100%) with the commercial RealStar® Malaria S&T PCR Kit 1.0 (100%). These results suggest that the multiplex malaria Pan/Pf/Pv/IC LAMP could be used as a point-of-care molecular diagnostic test for malaria.
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Gupta, Himanshu, Mohammed P. Afsal, Seema M. Shetty, Kapaettu Satyamoorthy, and Shashikiran Umakanth. "Plasmodium vivax infection causes acute respiratory distress syndrome: a case report." Journal of Infection in Developing Countries 9, no. 08 (2015): 910–13. http://dx.doi.org/10.3855/jidc.6813.
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Plasmodium falciparum (Pf) is associated with numerous complications and high mortality, whereas Plasmodium vivax (Pv) infection is generally considered to be benign. However, severe complications, such as acute respiratory distress syndrome (ARDS) in Pv infection, are emerging. This case report highlights the complication of ARDS during the course of Pv infection in a 60-year-old woman. The diagnosis of the patient was made using microscopy, immunochromatography, and polymerase chain reaction assays for Pf and Pv species. The data indicated the presence of mono-Pv infection in the patient’s blood, and Pf infection was specifically ruled out. The patient was discharged after intensive supportive care and antimalarial treatment. Pv infection is associated with ARDS and other complications such as sepsis and multi-organ dysfunction syndrome; this enhanced severity of Pv infection, if unrecognized, can lead to more deaths in malaria-endemic areas.
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Azam, Mudsser, Kirti Upmanyu, Ratan Gupta, et al. "Development of Two-Tube Loop-Mediated Isothermal Amplification Assay for Differential Diagnosis of Plasmodium falciparum and Plasmodium vivax and Its Comparison with Loopamp™ Malaria." Diagnostics 11, no. 9 (2021): 1689. http://dx.doi.org/10.3390/diagnostics11091689.
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To strengthen malaria surveillance, field-appropriate diagnostics requiring limited technical resources are of critical significance. Loop-mediated isothermal amplification (LAMP) based malaria diagnostic assays are potential point-of-care tests with high sensitivity and specificity and have been used in low-resource settings. Plasmodium vivax–specific consensus repeat sequence (CRS)-based and Plasmodium falciparum–specific 18S rRNA primers were designed, and a two-tube LAMP assay was developed. The diagnostic performance of a closed-tube LAMP assay and Loopamp™ Malaria Detection (Pan/Pf, Pv) kit was investigated using nested PCR confirmed mono- and co-infections of P. vivax and P. falciparum positive (n = 149) and negative (n = 67) samples. The closed-tube Pv LAMP assay showed positive amplification in 40 min (limit of detection, LOD 0.7 parasites/µL) and Pf LAMP assay in 30 min (LOD 2 parasites/µL). Pv LAMP and Pf LAMP demonstrated a sensitivity and specificity of 100% (95% CI, 95.96–100% and 89.85–100%, respectively). The LoopampTM Pan/Pf Malaria Detection kit demonstrated a sensitivity and specificity of 100%, whereas LoopampTM Pv showed a sensitivity of 98.36% (95% CI, 91.28–99.71%) and specificity of 100% (95% CI, 87.54–100%). The developed two-tube LAMP assay is highly sensitive (LOD ≤ 2 parasite/µL), demonstrating comparable results with the commercial Loopamp™ Malaria Detection (Pf/pan) kit, and was superior in detecting the P. vivax co-infection that remained undetected by the Loopamp™ Pv kit. The developed indigenous two-tube Pf/Pv malaria detection can reliably be used for mass screening in resource-limited areas endemic for both P. falciparum and P. vivax malaria.
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Ossè, Razaki A., Filémon Tokponnon, Germain Gil Padonou, et al. "Evidence of Transmission of Plasmodium vivax 210 and Plasmodium vivax 247 by Anopheles gambiae and An. coluzzii, Major Malaria Vectors in Benin/West Africa." Insects 14, no. 3 (2023): 231. http://dx.doi.org/10.3390/insects14030231.
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Current diagnostic and surveillance systems in Benin are not designed to accurately identify or report non-Plasmodium falciparum (Pf) human malaria infections. This study aims to assess and compare the prevalence of circumsporozoite protein (CSP) antibodies of Pf and P. vivax (Pv) in Anopheles gambiae s.l. in Benin. For that, mosquito collections were performed through human landing catches (HLC) and pyrethrum spray catches (PSC). The collected mosquitoes were morphologically identified, and Pf, Pv 210, and Pv 247 CSP antibodies were sought in An. gambiae s.l. through the ELISA and polymerase chain reaction (PCR) techniques. Of the 32,773 collected mosquitoes, 20.9% were An. gambiae s.l., 3.9% An. funestus gr., and 0.6% An. nili gr. In An. gambiae s.l., the sporozoite rate was 2.6% (95% CI: 2.1–3.1) for Pf, against 0.30% (95% CI: 0.1–0.5) and 0.2% (95% CI: 0.1–0.4), respectively, for Pv 210 and Pv 247. P. falciparum sporozoite positive mosquitoes were mostly An. gambiae (64.35%), followed by An. coluzzii (34.78%) and An. arabiensis (0.86%). At the opposite, for the Pv 210 sporozoite-positive mosquitoes, An. coluzzii and An. gambiae accounted for 76.92% and 23.08%, respectively. Overall, the present study shows that P. falciparum is not the only Plasmodium species involved in malaria cases in Benin.
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Gopalakrishnan, Nisha Thattamparambil, Supriya Papaiah, Smera Soman, and Krishnaraj Upadhyaya. "A Clinicopathological Study of Thrombocytopenia in Malaria Cases with Its Evaluation in Different Types of Malaria." Journal of Evolution of Medical and Dental Sciences 10, no. 33 (2021): 2707–11. http://dx.doi.org/10.14260/jemds/2021/553.
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BACKGROUND Malaria is a global health problem, caused by the protozoa plasmodium and is characterized by haematological abnormalities, with thrombocytopenia being the most common. Microscopic examination of thick and thin blood films is the gold standard in diagnosis of malaria. This study was conducted to assess the severity of thrombocytopenia in malaria patients and to correlate it with the type of malaria. METHODS A retrospective study was conducted in Yenepoya Medical College, Hospital, Mangalore for a period of 1.5 years. Patients of all ages who were hospitalized or attending OPD were included. Patients with dengue fever and drug-induced thrombocytopenia were excluded. Complete blood cell count was done using an automated cell count analyser. Thrombocytopenia was defined as a platelet count < 150,000 / μl. It was graded as severe: platelet count < 50,000/ μl, moderate: 50,000- 100,000/ μl and mild: 100,000-150,000 /μl. RESULTS Our study included 120 malaria positive cases with 102 (85 %) males and 18 (15 %) females. 90.8 % cases presented with thrombocytopenia, predominantly moderate to severe thrombocytopenia (80.7 %). Plasmodium vivax (Pv) was the most common species found in our study. Ninety-nine (82.5 %) cases were positive for Plasmodium vivax (Pv), 8 (6.6 %) cases for Plasmodium falciparum (Pf) and 13 (10.8 %) cases had mixed infection with both Plasmodium vivax and Plasmodium falciparum. Out of 99 cases which had vivax malaria, 88 (88.9 %) cases had thrombocytopenia. All 8 cases detected with falciparum malaria and 13 cases with mixed infection had thrombocytopenia. CONCLUSIONS The above findings can have therapeutic implications in avoiding unnecessary platelet infusion in malaria patients. Presence of thrombocytopenia in a patient with acute febrile illness can heighten suspicion of malaria, and initiate prompt treatment. KEY WORDS Thrombocytopenia, Malaria, Severity
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Vishruti Gandhi, Vishruti Gandhi, Prasad Muley, Niyati Parikh, Hardik Gandhi, and Akash Mehta. "Is rapid diagnostic test (malaria Pv/Pf Ag card test) reliable in diagnosing malaria." International Journal of Contemporary Pediatrics 5, no. 1 (2017): 92. http://dx.doi.org/10.18203/2349-3291.ijcp20175565.
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Background: Malaria is a protozoan disease transmitted by the bite of infected female anopheles mosquitoes is one of the most important parasitic diseases of human with transmission in 109 countries, affecting more than one billion people worldwide. This study was planned to compare the gold standard i.e. peripheral blood smear examination and the newer rapid diagnostic test (malaria plasmodium falciparum/ plasmodium vivax antigen card) to know the diagnostic accuracy of Rapid Diagnostic Test (RDT) kits. Methods: All the suspected cases of WHO defined malaria between 1month to 18 years of age were enrolled in the study.Results: Out of 96 clinically suspected cases of malaria 63 were confirmed by peripheral smear. The age range of participants ranged from 4 months to 17 years. On peripheral smear examination, out of 96 clinically suspected cases, 37 (38.5%) cases were positive for P. vivax, 23 (23.9%) were positive for P. falciparum and 3 (3.1%) were positive for both parasites by microscopy. Sensitivity and specificity of RDT for Plasmodium Vivax is 92.5% and 96.4% respectively. Sensitivity and specificity of RDT for Plasmodium Falciparum is 96.2% and 90%.Conclusions: The rational use of RDTs as a complement to microscopy might give substantial health benefits through earlier treatment, reduction in morbidity and mortality and more rationalized approach for choosing anti-malarial drugs, which in terms may prevent drug resistance.
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Kattenberg, Johanna Helena, Luis Cabrera-Sosa, Erick Figueroa-Ildefonso, et al. "Plasmodium vivax genomic surveillance in the Peruvian Amazon with Pv AmpliSeq assay." PLOS Neglected Tropical Diseases 18, no. 7 (2024): e0011879. http://dx.doi.org/10.1371/journal.pntd.0011879.
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Background Plasmodium vivax is the most predominant malaria species in Latin America, constituting 71.5% of malaria cases in 2021. With several countries aiming for malaria elimination, it is crucial to prioritize effectiveness of national control programs by optimizing the utilization of available resources and strategically implementing necessary changes. To support this, there is a need for innovative approaches such as genomic surveillance tools that can investigate changes in transmission intensity, imported cases and sources of reintroduction, and can detect molecular markers associated with drug resistance. Methodology/Principal findings Here, we apply a modified highly-multiplexed deep sequencing assay: Pv AmpliSeq v2 Peru. The tool targets a newly developed 41-SNP Peru barcode for parasite population analysis within Peru, the 33-SNP vivaxGEN-geo panel for country-level classification, and 11 putative drug resistance genes. It was applied to 230 samples from the Peruvian Amazon (2007–2020), generating baseline surveillance data. We observed a heterogenous P. vivax population with high diversity and gene flow in peri-urban areas of Maynas province (Loreto region) with a temporal drift using all SNPs detected by the assay (nSNP = 2909). In comparison, in an indigenous isolated area, the parasite population was genetically differentiated (FST = 0.07–0.09) with moderate diversity and high relatedness between isolates in the community. In a remote border community, a clonal P. vivax cluster was identified, with distinct haplotypes in drug resistant genes and ama1, more similar to Brazilian isolates, likely representing an introduction of P. vivax from Brazil at that time. To test its applicability for Latin America, we evaluated the SNP Peru barcode in P. vivax genomes from the region and demonstrated the capacity to capture local population clustering at within-country level. Conclusions/Significance Together this data shows that P. vivax transmission is heterogeneous in different settings within the Peruvian Amazon. Genetic analysis is a key component for regional malaria control, offering valuable insights that should be incorporated into routine surveillance.
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Balasubramanian, Sujata, Rifat S. Rahman, Chanthap Lon, et al. "Efficient Transmission of Mixed Plasmodium falciparum/vivax Infections From Humans to Mosquitoes." Journal of Infectious Diseases 221, no. 3 (2019): 428–37. http://dx.doi.org/10.1093/infdis/jiz388.
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Abstract Background In Southeast Asia, people are often coinfected with different species of malaria (Plasmodium falciparum [Pf] and Plasmodium vivax [Pv]) as well as with multiple clones of the same species. Whether particular species or clones within mixed infections are more readily transmitted to mosquitoes remains unknown. Methods Laboratory-reared Anopheles dirus were fed on blood from 119 Pf-infected Cambodian adults, with 5950 dissected to evaluate for transmitted infection. Among 12 persons who infected mosquitoes, polymerase chain reaction and amplicon deep sequencing were used to track species and clone-specific transmission to mosquitoes. Results Seven of 12 persons that infected mosquitoes harbored mixed Pf/Pv infection. Among these 7 persons, all transmitted Pv with 2 transmitting both Pf and Pv, leading to Pf/Pv coinfection in 21% of infected mosquitoes. Up to 4 clones of each species were detected within persons. Shifts in clone frequency were detected during transmission. However, in general, all parasite clones in humans were transmitted to mosquitoes, with individual mosquitoes frequently carrying multiple transmitted clones. Conclusions Malaria diversity in human hosts was maintained in the parasite populations recovered from mosquitoes fed on their blood. However, in persons with mixed Pf/Pv malaria, Pv appears to be transmitted more readily, in association with more prevalent patent gametocytemia.
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Marques, Rodolfo F., Alba Marina Gimenez, Eduardo Aliprandini, et al. "Protective Malaria Vaccine in Mice Based on the Plasmodium vivax Circumsporozoite Protein Fused with the Mumps Nucleocapsid Protein." Vaccines 8, no. 2 (2020): 190. http://dx.doi.org/10.3390/vaccines8020190.
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Plasmodium vivax is the most common species of human malaria parasite found outside Africa, with high endemicity in Asia, Central and South America, and Oceania. Although Plasmodium falciparum causes the majority of deaths, P. vivax can lead to severe malaria and result in significant morbidity and mortality. The development of a protective vaccine will be a major step toward malaria elimination. Recently, a formulation containing the three allelic variants of the P. vivax circumsporozoite protein (PvCSP—All epitopes) showed partial protection in mice after a challenge with the hybrid Plasmodium berghei (Pb) sporozoite, in which the PbCSP central repeats were replaced by the VK210 PvCSP repeats (Pb/Pv sporozoite). In the present study, the chimeric PvCSP allelic variants (VK210, VK247, and P. vivax-like) were fused with the mumps virus nucleocapsid protein in the absence (NLP-CSPR) or presence of the conserved C-terminal (CT) domain of PvCSP (NLP-CSPCT). To elicit stronger humoral and cellular responses, Pichia pastoris yeast was used to assemble them as nucleocapsid-like particles (NLPs). Mice were immunized with each recombinant protein adjuvanted with Poly (I:C) and presented a high frequency of antigen-specific antibody-secreting cells (ASCs) on days 5 and 30, respectively, in the spleen and bone marrow. Moreover, high IgG titers against all PvCSP variants were detected in the sera. Later, these immunized mice with NLP-CSPCT were challenged with Pb/Pv sporozoites. Sterile protection was observed in 30% of the challenged mice. Therefore, this vaccine formulation use has the potential to be a good candidate for the development of a universal vaccine against P. vivax malaria.
Book chapters on the topic "Plasmodium vivax (PV)"
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K. Quaye, Isaac, and Larysa Aleksenko. "Plasmodium vivax and Plasmodium ovale in the Malaria Elimination Agenda in Africa." In Current Topics and Emerging Issues in Malaria Elimination. IntechOpen, 2021. http://dx.doi.org/10.5772/intechopen.96867.
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In recent times, several countries in sub-Saharan Africa have reported cases of Plasmodium vivax (Pv) with a considerable number being Duffy negative. Current efforts at malaria elimination are focused solely on Plasmodium falciparum (Pf) excluding non-falciparum malaria. Pv and Plasmodium ovale (Po) have hypnozoite forms that can serve as reservoirs of infection and sustain transmission. The burden of these parasites in Africa seems to be more than acknowledged, playing roles in migrant and autochthonous infections. Considering that elimination and eradication is a current aim for WHO and Roll Back Malaria (RBM), the inclusion of Pv and Po in the elimination agenda cannot be over-emphasized. The biology of Pv and Po are such that the same elimination strategies as are used for Pf cannot be applied so, going forward, new approaches will be required to attain elimination and eradication targets.