01 February 2012: Basic Research
Lack of association of conjunctival MALT lymphoma with Chlamydiae or Helicobacter pylori in a cohort of Chinese patients
Ji-Ping Cai ABCDEF , Jin-Wei Cheng ABCDEF , Xiao-Ye Ma BCD , Yu-Zhen Li BCD , You Li BCD , Xiao Huang BCD , Rui-Li Wei AEFG
DOI: 10.12659/MSM.882462
Med Sci Monit 2012; 18(2): BR84-88
Background
MALT lymphoma is an extra-nodal marginal zone B cell lymphoma, and is the second most common inert tumor originating from mucosa-associated lymphoid tissue. There is definite evidence that occurrence of some B-cell lymphomas is associated with long-term chronic stimulation of microbials or autologous pathogens, which is most clearly exemplified by
Similar to the association of gastric MALT lymphoma with chronic stimulation of
The present study used the PCR method to detect
Material and Methods
MATERIAL:
Genomic DNA Mini Preparation Kit was purchased from MN NucleoSpin®, Germany. Tissue 740952 and Hotstart Taq were the products of TaKaRa DR028 (Dalian, China). All materials used, including tubes and pipette tips, were imported from AXYGEN.
METHODS:
Patient and sample collection: The study was approved by the local Ethics Review Board. Conjunctival MALT lymphoma specimens in the present study were from 14 patients (16 eyes) who were admitted at Shanghai Changzheng Hospital of the Second Military Medical University (Shanghai, China) between January 2008 and December 2009, all of whom were Han ethnicity and resided mainly in East China, without histories of keeping birds or having close contacts with birds. The patients included 9 males and 5 females who ranged in aged from 14 to 83 years, with a mean age of 55±16.76 years. Of the 2 patients with both eyes infected, both were female. The common presentation of the condition included the presence of subconjunctival (especially subfornical) pink tumors (salmon patch), whose course ranged from 3 months to 2 years. No history of lymphoma was elicited, nor was any tumor detected in another part of the body on physical examination. All patients received surgical treatment, and postoperative pathology and immunohistochemistry confirmed the diagnosis of MALT lymphoma in all patients. The tumor tissues, about 5mm in diameter, were obtained surgically, immediately washed with normal saline, stored in tubes and plunged directly in liquid nitrogen. The whole procedure was completed within 5 min. After 2–4 h preservation in liquid nitrogen, the 16 specimens were transferred to a −80°C freezer for preservation until later use.
GENOME EXTRACTION:
Genome extraction of the specimens was performed according to the manufacturer’s instructions. In brief, about 25 mg of freshly obtained MALT lymphoma tissue was cut off, digested in 180 μl T1 and 25 μl proteinase K at 56°C for 3 h, boiled in 200 μl B3 at 70°C for 10 min, and added to 210 μl ethanol. The mixture was put into the column, centrifuged at 11000g for 1 min, washed with 500 μl BW once, and again with 600 μl B5. The column was spun without loading for 1 min to dry the membrane, and was put into BE which had been preheated up to 70°C, and then centrifuged at 11,000g for 1 min. Purity of the extracted DNA was measured by spectrophotometry, and integrity was measured by electrophoresis.
PRIMER DESIGN AND SYNTHESIS:
The 16S rRNA sequences of C. psittaci, C. trachomatis, C. pneumoniae and H. pylori were from NCBI DataBank and the previous literature [16]. Primer design was according to microbial 16S rRNA gene sequences.
The above primers were synthesized by Shanghai Bioengineering Co., Shanghai, China.
DETECTION OF THE SPECIMENS:
We used 100 ng of tissue from each specimen as the template, and
PCR cycling of
Results
No
We observed that the electrophoretic bands of PCR amplification of specimens No. 8 and 16
Discussion
Research on the transformation of lymphocytes to cancer cells due to chronic microbial stimulation is of intense scientific interest world-wide. To confirm their correlation, it is necessary to detect the microorganisms in tumor tissues. In previous similar studies, DNA extraction was mostly from paraffin-embedded tumor pathologic specimens, and some of these tissues had been preserved for years before research; therefore, a portion of the DNA may have been degraded. The present study was a prospective study, different from previous reports in that the specimens used in the present study were freshly obtained from surgically resected and immediately frozen tumor tissues. Specimen collection and preservation were completed by the same person, thus minimizing DNA degradation and inter-specimen differences arising from personal influences, thereby maximizing the detection rate of the target DNA.
There is ample clinical and experimental evidence that
MALT lymphoma is the most common pathology in ocular adnexal lymphoma, accounting for 50–78% in developed countries [22–26], 80–90% in South Korea and Japan [27,28], and more than 80% in China [29–31]. Ocular adnexa include the eyelid, conjunctiva, orbit and lacrimal apparatus, of which the conjunctiva is most frequently exposed to the external environment directly, and therefore most susceptible to infection by microbial pathogens. If microbial infection is truly associated with ocular adnexal MALT lymphoma, the occurrence of the tumor is most likely to be related to chronic stimulation by exogenous microbials. Knowing that the incidence of conjunctival MALT lymphoma has been rising annually in recent years, we selected it as the subject of research in the present study, hoping to discover pathologic factors related to the etiology of the tumor in a limited number of cases. To our knowledge, this is the first study in China using fresh specimens of conjunctival MALT lymphoma from a cohort of Chinese patients to explore possible correlations between MALT lymphoma and microbial infections.
Italian researchers reported the presence of
Although we cannot deny possible errors and differences arising from specimen selection and detection methodology, the main problem is that we can neither rule out nor confirm the cause-effect relationship between them. In addition,
Conclusions
No
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