High-speed shaking of frozen blood clots for extraction of human and malaria parasite DNA
<p>Abstract</p> <p>Background</p> <p>Frozen blood clots remaining after serum collection is an often disregarded source of host and pathogen DNA due to troublesome handling and suboptimal outcome.</p> <p>Methods</p> <p>High-speed shaking of clot...
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doaj-c76483f6bcca46c483b2c1fb54df12e12020-11-24T22:00:04ZengBMCMalaria Journal1475-28752011-08-0110122910.1186/1475-2875-10-229High-speed shaking of frozen blood clots for extraction of human and malaria parasite DNAMohammed AdanLebbad MarianneMacharia AlexLundblom KlaraFärnert Anna<p>Abstract</p> <p>Background</p> <p>Frozen blood clots remaining after serum collection is an often disregarded source of host and pathogen DNA due to troublesome handling and suboptimal outcome.</p> <p>Methods</p> <p>High-speed shaking of clot samples in a cell disruptor manufactured for homogenization of tissue and faecal specimens was evaluated for processing frozen blood clots for DNA extraction. The method was compared to two commercial clot protocols based on a chemical kit and centrifugation through a plastic sieve, followed by the same DNA extraction protocol. Blood clots with different levels of parasitaemia (1-1,000 p/μl) were prepared from parasite cultures to assess sensitivity of PCR detection. In addition, clots retrieved from serum samples collected within two epidemiological studies in Kenya (n = 630) were processed by high speed shaking and analysed by PCR for detection of malaria parasites and the human α-thalassaemia gene.</p> <p>Results</p> <p>High speed shaking succeeded in fully dispersing the clots and the method generated the highest DNA yield. The level of PCR detection of <it>P. falciparum </it>parasites and the human thalassaemia gene was the same as samples optimally collected with an anticoagulant. The commercial clot protocol and centrifugation through a sieve failed to fully dissolve the clots and resulted in lower sensitivity of PCR detection.</p> <p>Conclusions</p> <p>High speed shaking was a simple and efficacious method for homogenizing frozen blood clots before DNA purification and resulted in PCR templates of high quality both from humans and malaria parasites. This novel method enables genetic studies from stored blood clots.</p> http://www.malariajournal.com/content/10/1/229 |
collection |
DOAJ |
language |
English |
format |
Article |
sources |
DOAJ |
author |
Mohammed Adan Lebbad Marianne Macharia Alex Lundblom Klara Färnert Anna |
spellingShingle |
Mohammed Adan Lebbad Marianne Macharia Alex Lundblom Klara Färnert Anna High-speed shaking of frozen blood clots for extraction of human and malaria parasite DNA Malaria Journal |
author_facet |
Mohammed Adan Lebbad Marianne Macharia Alex Lundblom Klara Färnert Anna |
author_sort |
Mohammed Adan |
title |
High-speed shaking of frozen blood clots for extraction of human and malaria parasite DNA |
title_short |
High-speed shaking of frozen blood clots for extraction of human and malaria parasite DNA |
title_full |
High-speed shaking of frozen blood clots for extraction of human and malaria parasite DNA |
title_fullStr |
High-speed shaking of frozen blood clots for extraction of human and malaria parasite DNA |
title_full_unstemmed |
High-speed shaking of frozen blood clots for extraction of human and malaria parasite DNA |
title_sort |
high-speed shaking of frozen blood clots for extraction of human and malaria parasite dna |
publisher |
BMC |
series |
Malaria Journal |
issn |
1475-2875 |
publishDate |
2011-08-01 |
description |
<p>Abstract</p> <p>Background</p> <p>Frozen blood clots remaining after serum collection is an often disregarded source of host and pathogen DNA due to troublesome handling and suboptimal outcome.</p> <p>Methods</p> <p>High-speed shaking of clot samples in a cell disruptor manufactured for homogenization of tissue and faecal specimens was evaluated for processing frozen blood clots for DNA extraction. The method was compared to two commercial clot protocols based on a chemical kit and centrifugation through a plastic sieve, followed by the same DNA extraction protocol. Blood clots with different levels of parasitaemia (1-1,000 p/μl) were prepared from parasite cultures to assess sensitivity of PCR detection. In addition, clots retrieved from serum samples collected within two epidemiological studies in Kenya (n = 630) were processed by high speed shaking and analysed by PCR for detection of malaria parasites and the human α-thalassaemia gene.</p> <p>Results</p> <p>High speed shaking succeeded in fully dispersing the clots and the method generated the highest DNA yield. The level of PCR detection of <it>P. falciparum </it>parasites and the human thalassaemia gene was the same as samples optimally collected with an anticoagulant. The commercial clot protocol and centrifugation through a sieve failed to fully dissolve the clots and resulted in lower sensitivity of PCR detection.</p> <p>Conclusions</p> <p>High speed shaking was a simple and efficacious method for homogenizing frozen blood clots before DNA purification and resulted in PCR templates of high quality both from humans and malaria parasites. This novel method enables genetic studies from stored blood clots.</p> |
url |
http://www.malariajournal.com/content/10/1/229 |
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