Cell line data – Leica Biosystems Bond Oracle HER2 IHC System User Manual

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Leica Biosystems Bond Oracle HER2 IHC System Instructions for Use TA9145 EN-CE-Rev_E 18/06/2013

Cell Line Data

Cell Line

BOND Oracle
HER2 IHC System
Profile

HER2
Receptor Load
per Cell*

HER2 Gene Amplification Status

+

HER2 Copy
Number

HER2:Chr17
Gene Ratio

SK-BR-3

3+

4.3x10

5

13.35

3.55

MDA-MB-453

2+

1.4x10

5

5.73

2.05

MDA-MB-175

1+

6.3x10

4

3.33

1.20

MDA-MB-231

0

9.3x10

3

3.15

1.13

*HER2 receptor load analysis as assessed by flow cytometry.

+

HER2 Gene Amplification Status as assessed by dual probe

(HER2:Chromosome 17) FISH.
Table 5. HER2 Control Slide profile

Clinical Concordance of Bond Oracle HER2 IHC System v Dako

HercepTest

Part one of the study examined the suitability of the Bond Oracle HER2 IHC System for use

as an aid in determination of treatment with Herceptin® (trastuzumab) therapy. The study was

designed to examine the concordance between the Bond Oracle HER2 IHC System and the

Dako HercepTest, considered as the ‘gold standard’ for this assay. The acceptance criterion

was defined as greater than 75% overall concordance between the two tests with a 95%

confidence interval (CI).
The study was conducted as a two-site, US based, blinded evaluation. Each investigational site

was supplied with formalin-fixed, paraffin-embedded breast cancer samples of known HER2

status. Cases were selected in reverse consecutive order from the clinical archives, representing

the consecutive flow of cases into a histopathology department for clinical testing, and tested

independently of other prognostic and/or predictive factors, with no bias introduced to the cohort.

Cohorts of 160 and 292 specimens were tested at Site 1 and Site 2 respectively. Each cohort

had an equal representation of equivocal/positive (2+, 3+) and negative (0, 1+) cases, based on

previously assigned HER2 IHC scores, resulting in a total study population of 452 samples.

Twelve samples were considered unsuitable, due to lack of sufficient invasive tumor and were

removed from the study. A further nine samples could not be scored as a result of tissue lifting

from the slide surface, resulting in a final study population of 431 samples.
All cases were stained with the HercepTest according to the manufacturer’s instructions as

specified in the package insert. Sequential sections from each case were stained with the Bond

Oracle HER2 IHC System on board an automated Leica Biosystems BOND fully automated,

advanced staining system. All cases were de-linked from unique patient identifying information

and were accompanied by clinical data relating to tumor size, tumor stage, tumor grade and

estrogen receptor status.
All stained slides were masked and scored in a randomized fashion by trained observers at

two sites. For 2x2 concordance analysis, scores were interpreted as negative if the staining

intensity was 0 or 1+, and positive for scores of 2+ or 3+. For 3x3 concordance analysis, scores

were interpreted as negative if the staining was 0 or 1+, equivocal for scores of 2+ and positive

for scores of 3+. Data was then analyzed for positive staining agreement and negative staining

agreement.