Lactococcus lactis expressing sand fly PpSP15 salivary protein confers long-term protection against Leishmania major in BALB/c mice

Davarpanah, Elaheh; Seyed, Negar; Bahrami, Fatemeh; Rafati, Sima; Safaralizadeh, Reza; Taheri, Tahereh

doi:10.1371/journal.pntd.0007939

Cited by 14 publications

(10 citation statements)

References 63 publications

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“…Notably, LJL-143 and LJM-17 were proposed as good vaccine candidates against canine Leishmaniasis caused by L. infantum, although an in vivo protective phenotype is yet to be demonstrated (Collin et al, 2009;Abbehusen et al, 2018). Additionally, from the saliva of the closely related P. duboscqui and P. papatasi sand flies, the homologous salivary proteins PpSP15 and PdSP15 (also known as PduM02) protected mice and non-human primates effectively from L. major-induced CL (Oliveira et al, 2008;Oliveira et al, 2015;Davarpanah et al, 2020). Three other proteins from the saliva of P. papatasi, PpSP36 (apyrase), PpSP42, and PpSP44 (both yellow-related proteins) were also proposed as good vaccine candidates for human CL (Tlili et al, 2018); however, efficacy results are either still missing, or contrary to this hypothesis in the case of PpSP44 in mice (Oliveira et al, 2008).…”

Section: Sand Fly Salivary Proteins As Anti-leishmania Vaccinesmentioning

confidence: 99%

“…interferon-g, and IL-12)/low anti-inflammatory (e.g. IL-4, IL-10, TGF-) CD4+ T cell-induced cytokine responses Gomes et al, 2008;Oliveira et al, 2008;Collin et al, 2009;Tavares et al, 2011;Xu et al, 2011;de Moura et al, 2013;Abi Abdallah et al, 2014;Oliveira et al, 2015;Abbehusen et al, 2018;Cunha et al, 2018;Tlili et al, 2018;Gholami et al, 2019;Cecilio et al, 2020;Davarpanah et al, 2020).…”

Section: Sand Fly Salivary Proteins As Anti-leishmania Vaccinesmentioning

confidence: 99%

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Some Good and Some Bad: Sand Fly Salivary Proteins in the Control of Leishmaniasis and in Autoimmunity

Aoki

Abdeladhim

et al. 2022

Front. Cell. Infect. Microbiol.

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Sand flies are hematophagous insects responsible for the transmission of vector-borne diseases to humans. Prominent among these diseases is Leishmaniasis that affects the skin and mucous surfaces and organs such as liver and spleen. Importantly, the function of blood-sucking arthropods goes beyond merely transporting pathogens. The saliva of vectors of disease contains pharmacologically active components that facilitate blood feeding and often pathogen establishment. Transcriptomic and proteomic studies have enumerated the repertoire of sand fly salivary proteins and their potential use for the control of Leishmaniasis, either as biomarkers of vector exposure or as anti-Leishmania vaccines. However, a group of specific sand fly salivary proteins triggers formation of cross-reactive antibodies that bind the ectodomain of human desmoglein 1, a member of the epidermal desmosomal cadherins. These cross-reactive antibodies are associated with skin autoimmune blistering diseases, such as pemphigus, in certain immunogenetically predisposed individuals. In this review, we focus on two different aspects of sand fly salivary proteins in the context of human disease: The good, which refers to salivary proteins functioning as biomarkers of exposure or as anti-Leishmania vaccines, and the bad, which refers to salivary proteins as environmental triggers of autoimmune skin diseases.

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Section: Sand Fly Salivary Proteins As Anti-leishmania Vaccinesmentioning

confidence: 99%

Section: Sand Fly Salivary Proteins As Anti-leishmania Vaccinesmentioning

confidence: 99%

Some Good and Some Bad: Sand Fly Salivary Proteins in the Control of Leishmaniasis and in Autoimmunity

Aoki

Abdeladhim

et al. 2022

Front. Cell. Infect. Microbiol.

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“…This recombinant strain have a great efficiency in inducing mucosal and systemic immune responses in chicken, against pathogenic avian influenza virus infection. Recently, alternative strategies to display the antigens at the L. lactis surface were developed, such as using a combination of Usp45 and the cA (C terminus of the peptidoglycan-biding domain) domain of the N-Acetyl-muraminidase [ 145 ], the Spax anchoring domain (Lei et al, 2020) or the PrtP signal peptide [ 161 ].…”

Section: Plasmid Vectors Available For Plasmid Dna and Recombinantmentioning

confidence: 99%

Plasmid Replicons for the Production of Pharmaceutical-Grade pDNA, Proteins and Antigens by Lactococcus lactis Cell Factories

Duarte

Monteiro

2021

IJMS

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The Lactococcus lactis bacterium found in different natural environments is traditionally associated with the fermented food industry. But recently, its applications have been spreading to the pharmaceutical industry, which has exploited its probiotic characteristics and is moving towards its use as cell factories for the production of added-value recombinant proteins and plasmid DNA (pDNA) for DNA vaccination, as a safer and industrially profitable alternative to the traditional Escherichia coli host. Additionally, due to its food-grade and generally recognized safe status, there have been an increasing number of studies about its use in live mucosal vaccination. In this review, we critically systematize the plasmid replicons available for the production of pharmaceutical-grade pDNA and recombinant proteins by L. lactis. A plasmid vector is an easily customized component when the goal is to engineer bacteria in order to produce a heterologous compound in industrially significant amounts, as an alternative to genomic DNA modifications. The additional burden to the cell depends on plasmid copy number and on the expression level, targeting location and type of protein expressed. For live mucosal vaccination applications, besides the presence of the necessary regulatory sequences, it is imperative that cells produce the antigen of interest in sufficient yields. The cell wall anchored antigens had shown more promising results in live mucosal vaccination studies, when compared with intracellular or secreted antigens. On the other side, engineering L. lactis to express membrane proteins, especially if they have a eukaryotic background, increases the overall cellular burden. The different alternative replicons for live mucosal vaccination, using L. lactis as the DNA vaccine carrier or the antigen producer, are critically reviewed, as a starting platform to choose or engineer the best vector for each application.

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“…Moreover, L. lactismediated delivery of DNA vaccines also lead to the expression of post-translationally modified antigens by host cells resulting in presentation of conformationally restricted epitopes to the immune system for induction of both cellular and humoral immune responses [112]. Also, with the aforementioned properties, the last two decades witnesses the use of genetically engineered L. lactis system as effective oral based vaccine vehicles for delivering antigens of viruses, bacteria and parasites to elicit both systemic and mucosal immunity [155][156][157][158]. Finally, the size of PV1A and PV3B recombinant DNA (obtained after insertion of cDNA into pIL1 expression vector) was observed as 7477 bp and 8377 bp, respectively which lies inside the ORF and could be translated into respective protein sequences with four additional amino acids (MCKC) at the N-terminus (Fig.…”

Section: Codon Optimization In Silico Cloning and Expression Of Pv1a And Pv3bmentioning

confidence: 99%

A cutting-edge immunoinformatics approach for design of multi-epitope oral vaccine against dreadful human malaria

Pritam

Singh

Swaroop

et al. 2020

International Journal of Biological Macromolecules

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Human malaria is a pathogenic disease mainly caused by Plasmodium falciparum, which was responsible for about 405,000 deaths globally in the year 2018. To date, several vaccine candidates have been evaluated for prevention, which failed to produce optimal output at various preclinical/clinical stages. This study is based on designing of polypeptide vaccines (PVs) against human malaria that cover almost all stages of life-cycle of Plasmodium and for the same 5 genome derived predicted antigenic proteins (GDPAP) have been used. For the development of a multi-immune inducer, 15 PVs were initially designed using T-cell epitope ensemble, which covered N99% human population as well as linear B-cell epitopes with or without adjuvants. The immune simulation of PVs showed higher levels of T-cell and B-cell activities compared to positive and negative vaccine controls. Furthermore, in silico cloning of PVs and codon optimization followed by enhanced expression within Lactococcus lactis host system was also explored. Although, the study has sound theoretical and in silico findings, the in vitro/in vivo evaluation seems imperative to warrant the immunogenicity and safety of PVs towards management of P. falciparum infection in the future.

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Lactococcus lactis expressing sand fly PpSP15 salivary protein confers long-term protection against Leishmania major in BALB/c mice

Cited by 14 publications

References 63 publications

Some Good and Some Bad: Sand Fly Salivary Proteins in the Control of Leishmaniasis and in Autoimmunity

Some Good and Some Bad: Sand Fly Salivary Proteins in the Control of Leishmaniasis and in Autoimmunity

Plasmid Replicons for the Production of Pharmaceutical-Grade pDNA, Proteins and Antigens by Lactococcus lactis Cell Factories

A cutting-edge immunoinformatics approach for design of multi-epitope oral vaccine against dreadful human malaria

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