Automatic identification of biological microorganisms using three-dimensional complex morphology

Seokwon Yeom; Bahram Javidi

doi:10.1117/1.2187017

1 March 2006 Automatic identification of biological microorganisms using three-dimensional complex morphology

Seokwon Yeom, Bahram Javidi

Author Affiliations +

Journal of Biomedical Optics, Vol. 11, Issue 2, 024017 (March 2006). https://doi.org/10.1117/1.2187017

Abstract

We propose automated identification of microorganisms using three-dimensional (3-D) complex morphology. This 3-D complex morphology pattern includes the complex amplitude (magnitude and phase) of computationally reconstructed holographic images at arbitrary depths. Microscope-based single-exposure on-line (SEOL) digital holography records and reconstructs holographic images of the biological microorganisms. The 3-D automatic recognition is processed by segmentation, feature extraction by Gabor-based wavelets, automatic feature vector selection by graph matching, training rules, and a decision process. Graph matching combined with Gabor feature vectors measures the similarity of complex geometrical shapes between a reference microorganism and unknown biological samples. Automatic selection of the training data is proposed to achieve a fully automatic recognition system. Preliminary experimental results are presented for 3-D image recognition of Sphacelaria alga and Tribonema aequale alga.

1. Introduction

Three-dimensional (3-D) as well as two-dimensional (2-D) optical and image processing techniques have been investigated to identify specific objects in unknown scenes. ^{1, 2, 3, 4, 5, 6, 7, 8, 9, 10, 11, 12, 13} Automatic and real-time identification of microorganisms has vast potential for various applications such as detection of biological weapons and harmful diseases, diagnosis of diseases, investigation of food safety, and ecological monitoring. There are conventional methods to identify microorganisms; however, the conventional techniques require time-consuming culturing and biochemical analysis with special skills. Therefore, automated and real-time recognition of microorganisms using 3-D optoelectronic imaging and can be beneficial.

Automated discrimination of living microorganisms in unknown images is very challenging. Tiny biological living objects can have simple and undistinguishable morphologies between different species; and many morphological variants exist in the same class.¹⁴ Research and development in this field have been performed using specific color and shapes based on captured 2-D intensity images.^{15, 16, 17, 18, 19, 20} The identification of tuberculosis bacteria and Vibrio cholerae has been studied based on their colors and 2-D shapes.^{15, 16} In Ref. 17, bacteria in a wastewater treatment plant are identified by morphological descriptors. The aggregation of streptomyces is classified into different phases by measuring the aggregation size and reaction time.¹⁸ In Ref. 19, plankton recognition is performed using preselected geometrical features. More research on image analysis and recognition of microorganisms can be found in Ref. 20. Recently, 3-D microorganism recognition was proposed using the single-exposure on-line (SEOL) digital holography.^{3, 13}

In this paper, complex information (magnitudes and phase) is utilized, providing distinct features that are impossible to be observed on 2-D intensity images. The phase change is due to the retardation of light as it propagates through the biological sample. We propose the automatic selection process of training data and present experimental results on the recognition of microorganisms. Figure 1 shows the block diagram of the recognition system. Microorganism in the Fresnel diffraction field is recorded by SEOL digital holography.^{11, 12, 13} Complex amplitude holographic images^{21, 22, 23, 24} are reconstructed at arbitrary depths by the inverse Fresnel transformation. The complex morphological pattern is segmented and salient features are extracted by the Gabor-based wavelets.^{25, 26} The training data is automatically selected by means of Gabor feature vectors and the graph matching technique.^{27, 28, 29, 30, 31} The automatic selection of training data is useful when biological samples overlap and∕or cluster, which make it difficult to select individual objects as training data. The rigid graph matching (RGM) techniques measures the similarity of complex geometrical shapes between a reference microorganism and unknown biological objects. A training rule is applied and the mean vector is stored into the database for the known reference. For the identification of unknown inputs, Euclidean distance between the reference mean vector and the feature vector of input objects are compared with a threshold.

Fig. 1

Block diagram of the automatic and real-time identification system.

Section 2 briefly reviews the recording and reconstruction of the SEOL digital holography. The segmentation and Gabor-based wavelets are illustrated in Sec. 3. Section 4 describes the feature vector selection with graph matching. Section 5 presents the training and decision processes. The experimental results and conclusions follow in Secs. 6, 7, respectively.

2. Review of SEOL Digital Holography

In this section, we review the recording and reconstruction of the 3-D complex information. The complex wave in the Fresnel diffraction field is recorded by the microscope-based Mach-Zehnder interferometer [see Fig. 2a ]. The 3-D complex holographic images are computationally reconstructed by the inverse Fresnel transformation at arbitrary depth $(d)$ [see Fig. 2b]. The SEOL digital holography is adopted for its advantages such as real-time detection and robustness to environmental fluctuation.¹³ The reconstruction process of the SEOL digital holography is described in Appendix A. Figure 3 shows the magnitude and the phase of the reconstructed holographic image of Sphacelaria alga.

Fig. 2

Schematic diagrams for (a) optical setup of SEOL digital holography and (b) the reconstruction process at arbitrary depth.

Fig. 3

Computationally reconstructed holographic image of Sphacelaria alga $(d = 180 mm)$ for (a) magnitude and (b) phase.

3. Segmentation and Feature Extraction

Since the coherent light is scattered by the semitransparent objects, the intensity on the foreground objects is lower than the background field. During the preprocessing, we subtract the background diffraction field in the reconstructed images. The detailed segmentation process is presented in Appendix B.

After the segmentation, features of microorganisms are extracted by the Gabor-based wavelets to generate a node vector at each pixel. Gabor-based wavelets are composed of multioriented and multiscaled Gaussian-form kernels that are suitable for local spectral analysis.^{25, 26} We define a node vector at the pixel $(m, n)$ as

Eq. 1

v (m, n) = {[\sum_{v = 1}^{V} ∣ h_{1 v} (m, n) ∣ \dots \sum_{v = 1}^{V} ∣ h_{U v} (m, n) ∣]}^{t},

Eq. 2

h_{u v} (m, n) = g_{u v} (m, n) * \hat{O} (m, n),

where

g_{u v} (x)

is the Gabor kernel with indices

u

and

v

;

U

and

V

are the total number of decompositions along the radial and tangential axes, respectively;

\hat{O}

is the segmented 3-D complex holographic image; ∗ stands for the 2-D convolution operator, and the superscript

t

denotes transpose. The kernel of the Gabor-based wavelets is presented in Appendix C.

4. Automatic Training Selection Using Graph Matching

In this section, we utilize the graph-matching technique to choose the data for the training process. The graph-matching technique was developed for pattern recognition of distorted objects.^{27, 28, 29, 30, 31} However, in the case that the image pattern of a reference object cannot be individually observed, or they are clustered as may be the case with some microorganisms, the selection of training data can be a labor-intensive task. In this paper, we achieve the fully automated recognition system by choosing the feature vectors to be trained by means of the RGM technique.

Let $R$ and $T$ be two identical and rigid graphs that are defined as sets of nodes associated in the local area. The graph $R$ and $T$ are placed on the image $O_{r}$ and the image $O_{t}$ of the same reference microorganism, respectively. The reference graph $R$ is translated by a fixed translation vector $p_{r}$ and rotated by a fixed clock-wise rotation angle $θ_{r}$ to cover a predetermined a referenced morphology. Therefore, the position vectors of the nodes in the reference graph $R$ are computed as

Eq. 3

x_{k} (p_{r}, θ_{r}) = A (θ_{r}) (x_{k}^{o} - x_{c}^{o}) + p_{r}, k = 1, \dots, K,

Eq. 4

A (θ) = [\begin{matrix} \cos θ & \sin θ \\ - \sin θ & \cos θ \end{matrix}],

where

x_{k}^{o}

is the position of the node

k

of a primitive graph without any translation and rotation,

x_{c}^{o}

is the center of the primitive graph, and

K

is the total number of nodes in the graph. In a similar way, any rigid motion of the training graph

T

on the image

O_{t}

can be described by a translation vector

p_{t}

and a clockwise rotation angle

θ_{t}

as

Eq. 5

x_{k} (p_{t}, θ_{t}) = A (θ_{t}) (x_{k}^{o} - x_{c}^{o}) + p_{t}, k = 1, \dots, K,

where

x_{k} (p_{t}, θ_{t})

is a position vector of the node

k

in the graph

T

.

We sequentially search for a similar local morphology with the referenced morphology on the image $O_{r}$ by translating and rotating the graph $T$ on the image $O_{t}$ . We choose the node vectors $v_{T} [x_{k} (p_{t}, θ_{t})]$ [see. Eq. 1] of the graph $T$ as training data if the following two conditions are satisfied:

Eq. 6

S_{R T} (p_{t}, {\hat{θ}}_{t}) > α_{S} and C_{R T} (p_{t}, {\hat{θ}}_{t}) < α_{C},

where

α_{S}

and

α_{C}

are thresholds for the similarity and the difference cost, and

{\hat{θ}}_{t}

is obtained by searching the best matching angle to maximize the similarity function at the position vector

p_{t}

as

Eq. 7

{\hat{θ}}_{t} = \underset{θ_{t}}{\arg \max} S_{R S} (p_{t}, θ_{t}) .

The similarity function and the difference cost in Eq. 6 are defined as

Eq. 8

S_{R T} (p_{t}, θ_{t}) = \frac{1}{K} \sum_{k = 1}^{K} \frac{⟨ v_{R} [x_{k} (p_{r}, θ_{r})], v_{T} [x_{k} (p_{t}, θ_{t})] ⟩}{∥ v_{R} [x_{k} (p_{r}, θ_{r})] ∥ ∥ v_{T} [x_{k} (p_{t}, θ_{t})] ∥},

Eq. 9

C_{R T} (p_{t}, θ_{t}) = \frac{1}{K} \sum_{k = 1}^{K} ∥ v_{R} [x_{k} (p_{r}, θ_{r})] - v_{T} [x_{k} (p_{t}, θ_{t})] ∥,

where ⟨∙⟩ stands for the inner product of two node vectors, and

v_{R} [x_{k} (p_{r}, θ_{r})]

is the node vector of the graph

R

.

5. Training and Decision Process

We define a feature vector as the collection of the node vectors of the graph. The feature vector to be trained is presented as

Eq. 10

f_{T} = {[v_{T}^{t} [x_{1} ({\hat{p}}_{t}, {\hat{θ}}_{t})] \dots v_{T}^{t} [x_{K} ({\hat{p}}_{t}, {\hat{θ}}_{t})]]}^{t},

where

v_{T} [x_{k} ({\hat{p}}_{t}, {\hat{θ}}_{t})]

is the node vector of the graph

T

, which is accepted for training; and the superscript

t

denotes matrix transpose. One common way for training and testing is to obtain the sample mean of training data and measure the Euclidean distance to determine the identity of unknown inputs. Let a set of training data be

Γ

:

Eq. 11

Γ = {f_{T}^{1}, \dots, f_{T}^{N_{T}}} .

The set

Γ

is composed of the feature vectors

f_{T}^{1}, \dots, f_{T}^{N_{T}}

, where

N_{T}

is the total number of the training data. We train those feature vectors by computing the sample mean as

Eq. 12

m_{f} = \frac{1}{N_{T}} \sum_{i = 1}^{N_{T}} f_{T}^{i} .

To recognize unknown inputs, the graph $S$ is translated and rotated on the unknown image $O_{s}$ as in the training procedure [see Eq. 5]. The graph $S$ has the same shape and size with the graph $R$ and $T$ . We compare the Euclidean distance with a threshold at every translation vector $p_{s}$ and the rotation angle ${\hat{θ}}_{s}$ . We accept the detection of the referenced 3-D complex morphology if the following condition is satisfied:

Eq. 13

∥ m_{f} - f_{S} (p_{s}, {\hat{θ}}_{s}) ∥ < α_{D},

where

α_{D}

is a threshold of detection. The feature vector

f_{S} (p_{s}, {\hat{θ}}_{s})

is obtained from the graph

S

, which is translated by the vector

p_{s}

and rotated by the angle

{\hat{θ}}_{s}

as

Eq. 14

f_{S} = {[v_{S}^{t} [x_{1} (p_{s}, {\hat{θ}}_{s})] \dots v_{S}^{t} [x_{K} (p_{s}, {\hat{θ}}_{s})]]}^{t},

and

{\hat{θ}}_{s}

is the angle, which minimizes Eq. 13 as

Eq. 15

{\hat{θ}}_{s} = \min_{θ_{s}} ∥ m_{f} - f_{S} (p_{s}, θ_{s}) ∥ .

6. Experimental Results

In the recording of the SEOL digital hologram,¹³ the size of the CCD for SEOL digital hologram is $2048 \times 2048 pixels$ and $1 pixel$ size is $9 \times 9 μ m$ . The CCD is placed $500 mm$ from the microorganism samples. The thickness of the microorganisms varies between 10 and $50 μ m$ . To test the recognition performance under various circumstances, we generate SEOL holograms of nine Sphacelaria alga and Tribonema aequale alga samples, respectively. We denote nine Sphacelaria samples as A1,…,A9 and nine Tribonema aequale samples as B1,…,B9. Since we have changed the position of the CCD during the experiments to test the robustness of the recognition system, the reconstruction depth for the focused image varies from $180 to 300 mm$ . After the reconstruction, the magnitude and phase information of computationally reconstructed holographic 3-D images are cropped and reduced into $256 ‐ \times 256 ‐ pixel$ images with a reduction ratio of 0.25 considering the computational complexity.

For the segmentation, we assume less than 20% of lower intensity region is occupied by microorganisms and the intensity of microorganisms is less than 45% of the background diffraction field. Therefore, the maximum intensity rate $r_{\max}$ in Eq. 18 and the segmentation probability $P_{s}$ in Eq. 19 are set at 0.45 and 0.2, respectively. The parameters for Gabor-based wavelets are set at $σ = π$ , $k_{0} = π ∕ 2$ , $δ = \sqrt{2}$ , $U = 5$ , and $V = 6$ in Appendix C. Figure 4 shows the component of the node vectors in Eq. 1.

Fig. 4

Components of the node vectors when (a) $u = 1$ , (b) $u = 2$ , (c) $u = 3$ , (d) $u = 4$ , and (e) $u = 5$ .

A rectangular grid is selected as a reference graph for the Sphacelaria alga, which shows regular thickness (see Fig. 3). The reference graph $R$ is composed of $25 \times 3$ nodes and the edge distance between nodes is $4 pixels$ in the $x$ and $y$ directions. Therefore, the total number of nodes in the graph is 75. The reference graph $R$ is placed with $p_{r} = {[81, 75]}^{t}$ and $θ_{r} = 135 \deg$ in the sample image A1. Considering the computational load, the graphs $T$ is translated by every $3 pixels$ in the $x$ and $y$ directions for measuring the similarity and difference to the graph $R$ for the training data selection. To search the best matching angles, the graph $T$ is rotated by $7.5 \deg$ from $0 to 180 \deg$ at every translated location. When the positions of rotated nodes are not integers, they are replaced with the nearest neighbor nodes. For the training data selection, the thresholds $α_{S}$ and $α_{C}$ are set at 0.95 and 1.2, respectively, in Eq. 6. For the decision process the threshold $α_{D}$ is set at 9.5 in Eq. 13. Figure 5a shows the reference graph on the sample image A1 and Fig. 5b shows automated selection of the training data where 33 graphs (feature vectors) are selected. Figures 5c and 5d show examples of recognition results performed on the true class sample A3, where 159 feature vectors are identified, and the false class sample B1, where no detection is accepted. Figure 6a shows the number of detection in true class samples A1 to A9 and false class samples B1 to B9. The number of detection varies from 14 to 159 in true class samples A1 to A9. No detection is accepted in false class samples B1 to B9. Figure 6b shows the minimum Euclidean distance in all samples. The minimum Euclidean distances in false class samples B1 to B9 are larger than those in true class samples A1 to A9 showing the discrimination capability of the proposed recognition system.

Fig. 5

(a) Reference graph on the sample A1, (b) training data selection on the sample A1, (c) decision result on true class sample A3, and (d) decision result on false class sample B1.

Fig. 6

(a) Number of detections and (b) minimum Euclidean distance.

7. Conclusions

In this paper, we have described the identification of biological microorganisms using their 3-D complex amplitude of geometrical information obtained by computer-reconstructed SEOL holographic images. ^{14, 32} Segmentation, Gabor feature extraction, feature vector selection using graph matching, and training and decision processes are presented to recognize a predetermined 3-D morphology in unknown biological samples. We choose the feature vectors to be trained by means of the RGM technique to remedy the possibility of biological samples overlap and∕or cluster, which make it difficult to select individual objects for the training purpose. Training and decision rules are applied to show the performance of the proposed system. Note that more sophisticated training and decision rules can be considered,^{7, 19} depending on the kind of microorganisms.

Appendices

Appendix A

The complex Fresnel diffraction field on microorganisms is reconstructed by the inverse Fresnel transformation at 3-D coordinates $(m, n, d)$ :

Eq. 16

O (m, n, d) = \exp [- j \frac{π}{λ d} (Δ X^{2} m^{2} + Δ Y^{2} n^{2})] \sum_{m^{'} = 1}^{N_{x}} \sum_{n^{'} = 1}^{N_{y}} H_{o} (m^{'}, n^{'}) \exp [- j \frac{π}{λ d} (Δ x^{2} m^{' 2} + Δ y^{2} n^{' 2})] \exp [j 2 π (\frac{m m^{'}}{N_{x}} + \frac{n n^{'}}{N_{y}})],

where

O (m, n, d)

is the complex amplitude reconstructed at 2-D discrete coordinates

(m, n)

and depth

d

;

H_{o}

is the SEOL digital hologram;

(Δ X, Δ Y)

and

(Δ x, Δ y)

are 2-D resolutions at the image plane and the hologram plane, respectively;

λ

is the wavelength of the coherent light source; and

N_{x}

and

N_{y}

are the size of the hologram in

x

and

y

directions, respectively.

Appendix B

Foreground objects are segmented by means of the histogram analysis of the background diffraction field:

Eq. 17

\hat{O} (m, n) = {\begin{cases} ∣ O (m, n) ∣ \exp {j [ϕ (m, n) - m_{ϕ}]} & if ∣ O (m, n) ∣ < I_{s} \\ 0 & otherwise \end{cases},

where

O (m, n)

is the complex holographic image

O (m, n) = ∣ O (m, n) ∣ \exp [j ϕ (m, n)]

, and

m_{ϕ}

is the sample mean of the phase

ϕ (m, n)

.

The threshold $I_{s}$ is determined from the histogram analysis and the maximum background field:

Eq. 18

I_{s} = \min {τ_{κ_{\min}} r_{\max} \max_{m, n} [∣ O (m, n) ∣]},

where

r_{\max}

is the maximum rate of the coherent light. The threshold

τ_{κ_{\min}}

is a minimum value of

τ_{κ}

satisfying the following equation:

Eq. 19

P_{s} ⩽ \frac{1}{N_{x} N_{y}} \sum_{i = 1}^{κ} h (τ_{i}),

where

P_{s}

is a predetermined segmentation probability;

h (τ_{i})

is the histogram, i.e., the number of pixels of which magnitude is between

τ_{i - 1}

and

τ_{i}

;

τ_{i}

is the

i

’th quantized magnitude level; and

κ_{\min}

is the minimum number of pixels that satisfies Eq. 19. In this paper, the total number of histogram levels is set at 256.

Appendix C

The discrete Gabor kernel $g_{u v} (m, n)$ at the position vector $x = {[m n]}^{t}$ is defined as

Eq. 20

g_{u v} (x) = \frac{{∣ k_{u v} ∣}^{2}}{σ^{2}} \exp (- \frac{{∣ k_{u v} ∣}^{2} {∣ x ∣}^{2}}{2 σ^{2}}) [\exp (j k_{u v}^{t} x) - \exp (- \frac{σ^{2}}{2})],

and the frequency response of the discrete Gabor kernel is

Eq. 21

G_{u v} (k) = 2 π {\exp (- \frac{σ^{2}}{2 {∣ k_{u v} ∣}^{2}} {∣ k - k_{u v} ∣}^{2}) - \exp [- \frac{σ^{2}}{2 {∣ k_{u v} ∣}^{2}} ({∣ k ∣}^{2} + {∣ k_{u v} ∣}^{2})]},

where

σ

is proportional to the standard deviation of the Gaussian envelope; and

k_{u v}

is a discrete wave number vector:

k_{u v} = k_{0 u} {[\cos ϕ_{v} \sin ϕ_{v}]}^{t}

,

k_{0 u} = k_{0} ∕ δ^{u - 1}

, and

ϕ_{v} = [(v - 1) ∕ V] π

, where

u = 1, \dots, U

and

v = 1, \dots, V

;

k_{0 u}

is the magnitude of the wave number vector;

ϕ_{v}

is the azimuth angle of the wave number vector;

k_{0}

is the maximum carrier frequency of the Gabor kernels;

δ

is the spacing factor in the frequency domain;

u

and

v

are the indices of the Gabor kernels;

U

and

V

are the total numbers of decompositions along the radial and tangential axes, respectively.

Acknowledgments

We are grateful to Inkyu Moon for supporting the experiments and the reconstruction on SEOL digital hologram.

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Seokwon Yeom and Bahram Javidi "Automatic identification of biological microorganisms using three-dimensional complex morphology," Journal of Biomedical Optics 11(2), 024017 (1 March 2006). https://doi.org/10.1117/1.2187017

Published: 1 March 2006

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KEYWORDS

Microorganisms

3D image processing

Holograms

Digital holography

3D image reconstruction

Image segmentation

Holography

1.

Introduction

Fig. 1

2.

Review of SEOL Digital Holography

Fig. 2

Fig. 3

3.

Segmentation and Feature Extraction

Eq. 1

Eq. 2

4.

Automatic Training Selection Using Graph Matching

Eq. 3

Eq. 4

Eq. 5

Eq. 6

Eq. 7

Eq. 8

Eq. 9

5.

Training and Decision Process

Eq. 10

Eq. 11

Eq. 12

Eq. 13

Eq. 14

Eq. 15

6.

Experimental Results

Fig. 4

Fig. 5

Fig. 6

7.

Conclusions

Appendices

Appendix A

Eq. 16

Appendix B

Eq. 17

Eq. 18

Eq. 19

Appendix C

Eq. 20

Eq. 21

Acknowledgments

References

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