PCR Characterization of Microbiota on Contracted and Non-Contracted Breast Capsules

Normal and contracted capsules were collected to investigate the microbiota on breast capsules. We included females who underwent implant replacement or removal for any reason. The subjects were treated according to the normal surgical procedures and received cefuroxime 1000 mg preoperatively. In all patients, the Baker score, as used in clinical practice [13], was determined by two physicians who together reached an agreement together. Baker scores of 1 and 2 were considered normal capsules, while Baker 3 and 4 were considered capsular contractures. The capsules were removed by the surgeon within the first 10 min of the operation using a cauterizer under sterile operating conditions. All capsules were taken at the site of incision at the inframammary fold. Special care was taken to avoid any contact of the capsules with the breast skin. A sample specimen (4 mm) was obtained from the removed capsules using a fresh, sterile scissor and tweezer at a sterile table. Afterwards, the specimens were collected in sterile specimen containers followed by immediate snap-freezing in liquid nitrogen and stored at − 20 °C until further analysis.

Females were included in the study who underwent reduction mammoplasty and had no history of prior breast surgery or a history of breast infection to investigate the microbiota of the glandular tissue. These females were treated according to normal surgical standards and received 1000 mg cefuroxime i.v. preoperatively. Before preparing the skin with chlorhexidine, a skin area of 3 × 3 cm was sampled with a swab (Copan flocked swab 552C moistened with 200 µl reduced transport fluid) at the site of incision. The breast tissue was removed by the surgeon under sterile operating conditions. A sample specimen (4 mm) was obtained from the glandular tissue using a fresh, sterile knife and tweezer at a sterile table. Both specimens were collected in sterile specimen containers and stored within two hours at -20 °C until further analysis. All samples were collected, stored and transported by one and the same investigator according to the aforementioned protocols.

Bacterial DNA was extracted from glandular breast tissue and capsule biopsy specimens by a first step consisting of lysis of bacteria. Biopsies measuring 4x4 mm were cut to pulp before adding 1 ml of easyMAG (BioMérieux, Marcy l′ Etoile, France) lysis buffer. This mixture was vortexed and incubated at room temperature while shaking at 1400 revolutions per minute (RPM) for 10 min. After a centrifugation step of 2 min at 14.000 RPM, the supernatant was used for DNA extraction on the easyMAG automated DNA isolation machine (BioMérieux). DNA was eluted in 70 µl NucliSens easyMAG extraction buffer 3 as provided by the manufacturer (BioMérieux), choosing the machine’s regular program with external lysis, according to the manufacturer’s instructions. Positive controls were added for each DNA isolation run. Amplification of IS-regions was performed with the IS-pro assay (IS-diagnostics, Amsterdam, the Netherlands) according to the protocol provided by the manufacturer. IS-pro differentiates bacterial species by the length of the 16S–23S rDNA intergenic spacer (IS) region with taxonomic classification by phylum-specific fluorescently labelled PCR primers (2). The procedure consists of two separate standard PCRs: the first PCR contains two different fluorescently labelled forward primers targeting different bacterial groups and three reverse primers providing universal coverage for those groups. The first forward primer is specific for the phyla Firmicutes, Actinobacteria, Fusobacteria and Verrucomicrobia (FAFV), and the second labelled forward primer is specific for the phylum Bacteroidetes. A separate PCR with a labelled forward primer combined with seven reverse primers is specific for the phylum Proteobacteria. Amplifications were carried out on a GeneAmp PCR system 9700 (Applied Biosystems, Foster City, CA). After PCR, 5 μl of PCR product was mixed with 20 μl formamide and 0.2 μl custom size marker (IS-diagnostics). DNA fragment analysis was performed on an ABI Prism 3500 Genetic Analyser (Applied Biosystems). Data were analysed with the IS-pro proprietary software suite (IS-Diagnostics, Amsterdam, the Netherlands), and the results are presented as microbial profiles. Automated species calling of IS-pro peaks was performed with the dedicated IS-pro software suite (IS-Diagnostics) in which peaks are linked to a database containing IS profile information of > 500 microbial species. Peaks lower than 128 relative fluorescence units (RFU) were regarded as background noise and were discarded from further analysis.

Data were further analysed with the Spotfire (TIBCO, Palo Alto, CA, USA) software package. Descriptive statistics are provided and presented as number (%) and mean (SD). Student’s t test was used for continuous data, and p values less than 0.05 were considered statistically significant. Statistical tests were performed using SPSS 22.0 (IBM SPSS Statistics for Windows, Version 22.0. IBM Corp., Armonk, NY, USA).

We included 50 breasts from 26 subjects. The breast capsules originated from cisgender females, with the exception of one male-to-female transgender subject. The mean age at the time of operation was 46 (SD 12.0) years. The primary indication for breast implantation was, in most cases, cosmetic (94%) and, in a few cases, for reconstructive surgery after breast cancer (6%). The Baker score was grade 1 in 12 cases, grade 2 in 16 cases, grade 3 in ten cases and grade 4 in 12 cases (see Table 1). The implants were removed after a mean of 11 (SD 5.6) years. The implantation duration for each Baker score was as follows: Baker 1: 6.6 years (SD 5.0 years), Baker 2: 11.5 years (SD 5.5 years), Baker 3: 8.8 years (SD 4.9 years) and Baker 4: 15.3 years (SD 4.0 years). This was significantly higher for higher Baker scores: Baker 1 vs. Baker 2 (p = 0.033), Baker 1 vs. Baker 4 (p = 0.002) and Baker 3 vs. Baker 4 (p = 0.017).

We included ten females receiving reduction mammoplasty due to breast hypertrophy. The mean age during operation was 51 (SD 7.4) years.

Both normal and contracted capsules were almost always sterile. In both groups, very low amounts of Staphylococcus spp. (S. epidermidis (4/50) and S. hominis (2/50)), Propionibacterium acnes (1/50) and Bacillus cereus (1/50) were detected (Fig. 1). There was no difference in bacterial presence between normal and contracted capsules (p = 1.0).

The skin of the breast mainly harboured Streptococcus spp. and Staphylococcus spp. while the glandular tissue of the breasts was sterile (Fig. 2).