CN54gp140 was formulated within the LSDFs for i.vag administration. Upon application the LSDFs boosted s.c.
Onalespib cell line primed mice indicating that the LSDFs reconsituted in vivo with the imbibing of vaginal fluid, resulting in intimate exposure of CN54gp140 with the mucosal-associated lymphoid tissue of the female genital tract. The LSDFs were conducive to long-term antigen storage stability. To the best of our knowledge this is the first description of lyophilized solid dosage forms as vaginal mucosal vaccine delivery modalities. This work was funded by a grant to St. George’s University of London, from the Bill and Melinda Gates Foundation and the Wellcome Trust, through the Grand Challenges in Global Health Initiative. We are indebted to Professors Wagner and Wolf, University of Regensburg, Germany and GENEART AG for access to CN54. “
“African swine fever (ASF) is a highly contagious, haemorrhagic
disease of pigs caused by a large, cytoplasmic, icosahedral DNA virus (ASFV) with a genome size of 170–193 kbp. Virulent isolates kill domestic pigs within 7–10 days of infection. In chronic cases ASF causes respiratory disorders and in some cases swelling around the leg joints and skin lesions. Domestic pigs can survive infection with less virulent isolates and in doing so can gain immunity to subsequent challenge with related virulent viruses [1], [2], [3], [4] and [5]. ASF is endemic in many sub-Saharan African countries as well as in Sardinia. In 2007 ASF was introduced into Georgia and from there spread rapidly to neighbouring countries PD0325901 in vivo in the Trans Caucasus
region, including Southern European Russia [6]. The virus has continued to spread through the Russian Federation and 18 federal subjects have reported outbreaks (OIE WAHID). Virus has also been isolated a number of times from wild boar in this region and the presence of ASF in this wildlife population is likely to make eradication more difficult [6]. Genotyping of ASFV isolates by partial sequencing of the B646L gene encoding the major capsid protein p72 has identified up to 22 genotypes [7] and [8]. Many of these are circulating in the long-established sylvatic cycle involving soft ticks of Ornithodoros spp. and warthogs in eastern and southern Africa. In many regions the isolates circulating in domestic pigs are genetically more similar. Previous work has shown Phosphoprotein phosphatase that pigs are protected from challenge with related virulent isolates following infection with natural low virulence isolates and with virus attenuated by passage in tissue culture or by deletion of genes involved in virulence [2], [3], [9] and [10]. Protection induced by the non-virulent OURT88/3 isolate was shown to require CD8+ T cells since depletion of these cells was shown to abrogate this protection [11]. Passive transfer of antibodies from pigs protected following infection with lower virulence isolates was also shown to protect naïve pigs from challenge with related virulent virus [12].
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