Patent Grant
9041792
In a first aspect, the invention relates to a method of generating a multicolour image of an unstained biological specimen, the specimen comprising at least two chemically different substances of interest.
In a second aspect, the invention relates to a data carrier.
In a third aspect, the invention relates to a system for generating a multicolour image of an unstained biological specimen, the object comprising at least two chemically different substances of interest.
In histopathology and cytopathology a pathologist routinely analyses microscopic images taken from tissues or cell smears. The specimens are typically analysed with a standard microscope using visible light. Due to the fact that cells and tissues hardly absorb visible light it is a common practice to stain the specimens. The staining chemical can be observed in visible light. It indicates the presence and generally also the amount of the structure it typically binds to. During many years of training and experience a pathologist learns how to interpret the stained images of specimens and to come to a diagnosis. In the digital pathology community the use of staining chemicals is generally considered mandatory for imaging slide samples in transmission.
Which staining method is chosen typically depends on the specific structure the pathologist is interesting in. A very popular staining method is the hematoxylin and eosin (H&E) stain. The hematoxylin binds to basophilic structures and colours them with a blue-purple hue. Basophilic structures are, for example, those cell components which contain nucleic acids and the cytoplasmic regions rich in RNA. Eosinophilic structures are generally composed of intracellular or extracellular protein and are coloured pink by the eosin.
However, staining has several major disadvantages. One of them is that the colour rendering in image of a stained specimen strongly depends on the stain method that has been used. The quality of the staining is not constant, as pointed out by T. Abe et al (T. Abe et al, “Colour Correction of Pathological Images Based on Dye Amount Quantification”. Optical Review, Vol. 12, No. 4, 2005, pp. 293-300). Yet a good quality is important for enabling the pathologist to come to a proper diagnosis. Another problem is related to the transfer of traditional pathology to automated diagnosis, which is an important development today. Quality variations observed among hospitals or even among staining machines or in staining machines over time present a serious hurdle for automated diagnosis. Different solutions have been proposed in order to solve these problems, such as improving the control of the staining process or by digitally correcting the multicolour image of the stained sample by means of a computer (see the above-mentioned article by T. Abe et al).
It is an object of the invention to provide a way of generating a multicolour image of an unstained biological specimen which does not require staining the specimen.
This object is achieved by the features of the independent claims. Further specifications and preferred embodiments are outlined in the dependent claims.
According to the first aspect of the invention, the method comprises
The specimen may be substantially transparant for visible light, having a transmissivity of, for example, more than 80%, or of more than 90%. The specimen may be a histopathological specimen, and it may be arranged on a microscope slide.
Generating the multicolour image on the basis of the substance images may comprise
At least one of the substances of interest may be assigned a colour that matches the colour of a dye capable of binding to that substance. More specifically, it is proposed to
The specimen may comprise as a first substance of interest protein and as a second substance of interest nucleic acid. The protein may be assigned a red or pink colour, and the nucleic acid may be assigned a blue, violet, or purple colour.
The multicolour image may be obtained from the superimposed single-colour images according to a subtractive colour model. That is, each of the colours assigned to the various substances of interest acts as a filter transmitting only the assigned colour. The multicolour image may then be produced by superimposing the single-colour images on a white background. Superimposing, for example, blue and red would produce a grey tone or black, rather than purple. Thereby the resemblance of the multicolor image to a conventional staining-based image can be improved.
The steps of converting and of superimposing may be performed on a computer.
Converting each substance image into a single-colour image may comprise
Generating the multicolour image on the basis of the substance images may comprise
The transmitted light image may be computed using the Beer-Lambert law with, as input data, the substance images and the postulated absorption spectra.
The substance images may be determined by
The substance images may be derived from the ultraviolet images using the Beer-Lambert law. This will be outlined in greater detail below.
According to the second aspect of the invention, a data carrier carries instructions for instructing a computer to control or to perform the method summarized above. The computer may be a PC or any other suitable information processing device or electronic controller.
According to the third aspect of the invention, the system for generating a multicolour image of the unstained specimen comprises
The optical system may comprise a microscope. The microscope may serve for both illuminating the specimen and for collecting light from the specimen. The microscope may be a conventional optical microscope or a scanning microscope.
Unless specified otherwise, identical or similar reference numerals appearing in different Figures label identical or similar components.
I(ν,z)=I0(ν)exp(−σ1(ν)(N1(z)−σ2(ν)N2(z))
where σ1(ν) and σ1(ν) are the absorption cross sections (in square meters, for example) of the first substance and of the second substance, respectively, and N1(z) and N2(z) are the numbers of particles per unit area on the axis between the positions 0 and z, of the first substance and of the second substance respectively. More precisely, N1(z) and N2(z) are the numbers of particles having a projection along the z-direction on that unit area, divided by the unit area. The 0 position is chosen on the upper surface 14. The z value is chosen to correspond to the lower surface 16 and will be suppressed from now on. Instead we introduce the dependence on x and y, that is, on the position in the x-y-plane 2, 4:
I(ν,x,y)=I0(ν,x,y)exp(−σ1(ν)(N1(x,y)−σ2(ν)N2(x,y)).
Evaluating the above relation for the two ultraviolet frequencies ν1 and ν2 yields a linear system for the numbers of particles per unit area, N1(x, y) and N2(x, y), of the first substance and of the second substance, respectively:
In the present application, the functions N1(x, y) and N2(x, y) are referred to as substance images since they provide an image of the distribution of the respective substance on a surface (in the present case, the lower surface 16 of the specimen 12). They can be represented graphically in different manners, for example, as shaded single-colour images, as contour plots, or as a surface defined on the x-y-plane. The transmitted intensity values I(ν1, x, y) and I(ν2, x, y), normalized by incident intensity values I0(ν1, x, y) and I0(ν2, x, y), form the ultraviolet images mentioned above. They are obtained by measuring the intensity of the incident ultraviolet light and the intensity of the transmitted ultraviolet light for various positions in the x y-plane and possibly interpolating between neighbouring positions. The cross sections σ1(ν1), σ2(ν1), σ1(ν2), σ1(ν2) are assumed to be known. For example, optimal/normalized spectral absorption coefficients of hematoxylin and eosin have been published by Abe et al (see the above-mentioned article). The substance images N1(x, y) and N2(x, y) are then derived by solving the linear system given above. The approach can readily be generalized to more than two substances. In order to determine a substance image for each of M substances in the specimen 12, the specimen 12 is successively illuminated M times, each time using light of a different frequency.
Schematically represented in
In
Referring now to
While the invention has been illustrated and described in detail in the drawings and in the foregoing description, the drawings and the description are to be considered exemplary and not restrictive. The invention is not limited to the disclosed embodiments. Equivalents, combinations, and modifications not described above may also be realized without departing from the scope of the invention.
The verb “to comprise” and its derivatives do not exclude the presence of other steps or elements in the matter the “comprise” refers to. The indefinite article “a” or “an” does not exclude a plurality of the subjects the article refers to. It is also noted that a single unit may provide the functions of several means mentioned in the claims. The mere fact that certain features are recited in mutually different dependent claims does not indicate that a combination of these features cannot be used to advantage. Any reference signs in the claims should not be construed as limiting the scope.
| Number | Date | Country | Kind |
|---|---|---|---|
| 08305854 | Nov 2008 | EP | regional |
| Filing Document | Filing Date | Country | Kind | 371c Date |
|---|---|---|---|---|
| PCT/IB2009/055159 | 11/19/2009 | WO | 00 | 5/26/2011 |
| Publishing Document | Publishing Date | Country | Kind |
|---|---|---|---|
| WO2010/061319 | 6/3/2010 | WO | A |
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| Number | Date | Country | |
|---|---|---|---|
| 20110228072 A1 | Sep 2011 | US |
