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Chinese Journal of Diagnostics(Electronic Edition) ›› 2014, Vol. 02 ›› Issue (04): 270-274. doi: 10.3877/cma.j.issn.2095-655X.2014.04.007

Special Issue:

• Basic Study • Previous Articles     Next Articles

Diagnosis of plasmodium malariae infection by nested PCR

Jin Li1, Chao Xu1, Qingkuan Wei1, Ting Xiao1, Xiangli Kong1, Yongbin Wang1, Benguang Zhang1, Yanbin Wei1, Changlei Zhao1, Bingcheng Huang1,()   

  1. 1. Shandong Academy of Medical Sciences, Shandong Institute of Parasitic Diseases, Shandong Provincial Reference Laboratory for Malaria Diagnosis, Jining 272033, China
  • Received:2014-02-16 Online:2014-11-26 Published:2014-11-26
  • Contact: Bingcheng Huang
  • About author:
    Corresponding author: Huang Bingcheng, Email:

Abstract:

Objective

To diagnose the imported plasmodium malariae cases with nested-PCR amplification of 18SSUrRNA gene.

Methods

Plasmodium DNA was extracted from anticoagulant blood as template with the plasmodium gene-specific primers in the first round of amplification, then the products of the first round were amplified as the second round template.The results of different subgroups of plasmodium were acquired.The target fragment of PCR was used for species identification and sequencing, comparing with the control sample of P. vivax and P. falciarum.

Results

By using the plasmodium gene-specific primers amplification, the fragments were amplified from the three samples with 1 200 bp.By using the interspecific primers amplification, specific fragments were amplified from the blood samples of P. vivax and P. falciarum with 120 bp and 205 bp respectively, and 144 bp from the suspicious patient with P. malariae specific primers.The suspicious patients did not have the specific fragment of P. ovale.The product of the suspicious patients was sequenced and compared with standard sequence registered in Genbank by blast.The comparison results showed that the fragment size and product sequence were in accordance with the reference.The results showed that nested PCR was more objective than the traditional microscopic examination.

Conclusions

The results indicate that nested PCR can be used to detect plasmodium with high specificity and identify plasmodium at the species level when microscopy is equivocal.The specific primers to amplify 18 SSUrRNA gene fragment can be used to diagnose plasmodium malariae infection.

Key words: Plasmodium malariae, Ribosome subunits, RNA, ribosomal, Polymerase chain reaction, nested, Diagnosis

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