Millennium/Empower

Advance Training for Teva

Dr. Shulamit Levin

levins@medtechnica.co.il

Reviewing Data

Review Multiple Channels

The list of channels is in the 2D channels view

The results of the integration and calculation will

be the Peaks view

A channel is a real original raw data

The list of results selected for review is shown

in the 2D Channels

The results of the integration and

calculation is in the Peaks view

All Reviews Windows

The Processing Methods Window

The Result
Results Window

Integrating
Complex Chromatograms

A Complex Chromatograms
1.00

0.80

AU

0.60

0.40

0.20

0.00
0.00

5.00

10.00

15.00

20.00

25.00

30.00
35.00
Minutes

40.00

45.00

50.00

55.00

60.00

65.00

Integrating Complex Chromatograms

0.030
0.025

ZOOM

0.020

AU

0.015
0.010
0.005
0.000
-0.005
-0.010
5.00

10.00

15.00

20.00

25.00

30.00

35.00

40.00

45.00

50.00

55.00

60.00

Minutes

0.004

ZOOM MORE

0.002

AU

0.000

-0.002

-0.004

-0.006
2.00

4.00

6.00

8.00

1 0.00 12.00 14.00 16.00 18.00 20.00 22.00 24.00 26.00 28.00 30.00 32.00 34.00 36.00 38.00 40.00 42.00 44.00 46.00 48.00 50.00
Minutes

Integrating Complex Chromatograms

Scaling Options

A Complex Chromatograms
Where to begin?

22.762

19.940

-0.006

24.890

23.526

24.215

22.380
22.478

20.837

-0.004

19.521

AU

-0.003

-0.005

22.082

21.275

-0.002

21.885

-0.001

21.594

21.111

Integrating Complex Chromatograms

Integration Events

-0.007
20.50

21.00

41.001

23.50

24.00

24.50

25.00

44.787

-0.005

-0.006

23.00

42.275

41.784

41.363

-0.004

40.438

AU

-0.003

22.50
Minutes

41.536
41.653

-0.002

22.00

42.459

41.995

-0.001

21.50

45.631

20.00

43.682

19.50

-0.007
40.50

41.00

4 1.50

42.00

42.50

43.00
Minutes

43.50

44.00

44.50

45.00

45.50

46.00

Integrating Complex Chromatograms

Setting Up The Components in the Component Table

Clear integration, then select

manually the major peaks, go
to The Processing Method
view and use:
OptionsOptions->
Fill from results

Integrating Complex Chromatograms

Setting Up The Components in the Component Table

Integrating Complex Chromatograms

Setting Up The Components in the Component Table

Integrating Complex Chromatograms

Setting Up The Components in the Component Table

Integrating Complex Chromatograms

Use: Show Components and Show Events

Integrating Complex Chromatograms

10

Integrating Complex Chromatograms

Inhibit Integration

Integrating Complex Chromatograms

Select a small narrow peak and get Peak width and

Threshold

ZOOM

0.004

0.002

AU

0.000

-0.002

-0.004

-0.006
2.00 4.00 6.00 8.00 10.00 12.00 14.00 16.00 18.00 20.00 22.00 24.00 26.00 28.00 30.00 32.00 34.00 36.00 38.00 40.00 42.00 44.00 46.00 48.00 50.00
Minutes

11

Integrating Complex Chromatograms

0.008
0.006
0.004

AU

0.002
0.000
-0.002
-0.004
-0.006
-0.008
28.00

28.50

29.00

29.50

30 .00

30.50

31.00

31.50

32.00

32.50

33.00

Minutes

0.010

0.006
0.004

31.140

29.345

0.008

0.000

31.795

AU

0.002

-0.002
-0.004
-0.006
-0.008
-0.010
28.40

28.60

28.80

29.00

29.20

29.40

29.60

29.80

30.00

30.20

30.40
30.60
Minutes

30.80

31.00

31.20

31.40

31.60

31.80

32.00

32.20

32.40

32.60

22.762

19.940

-0.006

24.890

23.526

24.215

22.380
22.478

20.837

-0.004

19.521

AU

-0.003

-0.005

22.082

21.275

-0.002

21.885

-0.001

21.594

21.111

Integrating Complex Chromatograms

Integration Events

-0.007
20.50

21.00

41.001

23.50

24.00

24.50

25.00

44.787

-0.005

-0.006

23.00

42.275

41.784

41.363

-0.004

40.438

AU

-0.003

22.50
Minutes

41.536
41.653

-0.002

22.00

42.459

41.995

-0.001

21.50

45.631

20.00

43.682

19.50

-0.007
40.50

41.00

4 1.50

42.00

42.50

43.00
Minutes

12

43.50

44.00

44.50

45.00

45.50

46.00

-0.006

40.50
41.00
4 1.50

7.880

-0.002

42.00

20.00

42.50

25.00

43.00
Minutes

30.00
Minutes

-0.005

43.50

13
44.00

29.345
31.140

35.00
40.00

44.50

45.00

45.00
45.50

51.650
51.851
52.471

36.948
37.619
38.241
38.590
38.844
39.758
40.051
40.180
40.408
40.544
41.444
41.756
42.129
42.553
42.761
42.910
43.073
43.331
43.911
44.214
44.898
46.679
47.320
47.611
48.154
48.507
48.865
49.680

31.795
33.070
33.788
34.140
34.565
34.950
35.388

0.015

21.905
22.507

23.081
23.340
24.210

0.025

26.048
26.920

4.820

0.030

45.631

15.00

42.460

10.00

44.787

-0.001

41.995

-0.005

12.226
12.393
12.708
13.590
13.881
15.617
15.980
16.199
16.163
16.984 17.382
18.853
19.869
20.250
20.513
20.775
21.280
21.429
22.332
23.848

0.000

41.657

41.532

5.00

43.682

-0.004

41.357

0.005

5.849

AU
0.010

41.003

40.438

AU

Integrating Complex Chromatograms

Just from Peak Width, Threshold & Inhibit Integration

0.020

50.00

Valey to Valey
Integrating Complex Chromatograms

-0.003

-0.007
46.00

55.00

Integrating Complex Chromatograms

Manual Exponential Skim

Integrating Complex Chromatograms

Height Rejection How to do it right

0.0012
0.0010
0.0008
0.0006

AU

0.0004
0.0002
0.0000
-0.0002

For peak width and Threshold

-0.0004
-0.0006
2.00

4.00

6.00

8.00

10.00

12.00

14.00

16.00

18.00 20.00
Minutes

14

22.00

24.00

26.00

28.00

30.00

32.00

34.00

36.00

5.831

16.818
17.635

Integrating Complex Chromatograms

Height Rejection How to do it right

0.0012

0.0000

35.644
35.820
35.953
36.314
36.693
37 375

15.228

12.115
13.181

0.0002

8.090
8.995

AU

0.0004

1.807
2.288
3.413
3.731
4.885
5.231
5.357
6.567

0.0006

30.297
31.148

0.0008

33.056

16.170

0.0010

-0.0002
-0.0004
-0.0006
2.00

4.00

6.00

8.00

10.00

12.00

14.00

16.00

18.00 20.00
Minutes

22.00

24.00

26.00

28.00

30.00

32.00

34.00

5.831

Integrating Complex Chromatograms

Height Rejection How to do it right

0.0003

8.995
8.090

0.0000

6.567

5.231
5.357

4.885

3.731

3.413

AU

1.807

0.0001

2.288

0.0002

-0.0001

-0.0002

1.00

1.50

2.00

2.50

3.00

3.50

4.00

4.50

5.00

5.50 6.00
Minutes

6.50

7.00

7.50

8.00

A segment in the chromatogram:

Some of them are not peaks

15

8.50

9.00

9.50

10.00

10.50

36.00

Height Rejection: h> 3x baseline noise

Baseline Start Time and

Baseline End Time
Noise (maximum voltage change over a 30-second interval). Noise value is a number of 30second intervals as determined by the % Run Time Over Which to Average parameter
The software determines the 30-second intervals by counting from the Baseline Start Time and the
Baseline End Time toward the middle of the chromatogram.
If the averaged region is < 30 seconds, noise is reported as a blank.
.

Condition
Total Run Time
% of Run Time to Average
Average Time
Baseline Start
Baseline End

Setting
10 minutes
5%
0.5 minute (5% of 10 minutes)
1 minute
9 minutes

System Suitability

16

Signal (Peak Height) to Noise

Must use System Suitability and Custom Fields***

Equation to use to calculate Signal/Noise:
Height/(1000*Baseline Noise)
(same injection for noise and peak for s/n calculation)
Modifications to this calculation:
Using different sample to calculate signal to noise
(Height/1000)/S0101.1.2487(Baseline_Noise) where S0101 is the Sample
Sample
label, 1 is the injection number and 2487channel1 is the Channel Name)
*** - Covered in the custom fields section

Detector Noise and Drift (ASTM)

Specify a time to calculate noise and drift results. For averaged noise/drift values, specify a
segment width (in seconds) for the software to divide the data into segments and averages for
each segment.
The noise and drift chromatogram results include: Total Values Detector Noise, Peak to Peak
Noise, and Detector Drift
Average Values Average Detector Noise, Average Peak to Peak Noise, and Average Detector
Drift

Only Detector Noise

17

Baseline Noise is in the Results Window

0.009x1000=9 uV
Minimum Height can be : 27

Baseline Noise is in the Results Window

1.24x10-4
1.23x10-4
1.22x10-4
1.21x10-4

AU

1.20x10-4
1.19x10-4
1.18x10-4
1.17x10-4
1.16x10-4
1.15x10-4
1.14x10-4
22.60

22.70

22.80

22.90

23.00

23.10

23.20
Minutes

~1x10-5 AU

18

23.30

23.40

23.50

23.60

23.70

Integrating Complex Chromatograms

Simple Processing Using the

Processing Wizard

Pre-enter the amounts in Run

Samples or Alter Sample for the
standard even for Internal Standard
Always select low concentration
standards/unknwons when using the
wizard to create a Processing Method
Recommended to select an unknown
to edit/test
Save the processing method, batch
process using the Sample Set,
Injections or Channel View
(If using the Injection/Channel view,
make sure to select Standards before
unknowns)

19

1. Peak Width used for Data Bunching

2. Threshold for Peak Detection

4. Minimum Area/Height for Peak Rejection

3. Peak Width used for Inhibit Integration

5. Calibration General

6. Component Names

*Injection Volumes for concentration

If a standard was selected, the component

names displayed in the drop down box is from
the names entered in the Amounts table in Run
Samples or Alter Sample

**Recommended for Linear 3 standard

concentrations, 3rd order 5
concentrations, etc.

*
**

20

7. Default Amounts

8. External or Internal Calibration

Ignore unless using Single Point

Calibration through Zero

For internal standard, select the component

desired (names will be displayed from the
entries in step # 6 of the wizard).

Use Run Sample Amounts or Default

Amounts from the Processing Method
view

**

9. Method Name is the processing

method
*Regulated customers must enter in a
comment

10. View the wizard results for the standard

Select the peaks tab and verify all desired peaks
are identified.

21

11. Method Name is the processing

method
*Regulated customers must enter in a
comment

12. View the wizard results for the standard

Select the Peaks tab and verify all desired
peaks are identified.

13. Verify peak Integration

14. Verify peak identification

Select a 2nd standard and click the

Integrate button.

Select the Calibrate. Make sure all desired

peaks are properly IDed.

22

15. Modify the acquisition Method Set to include the newly created processing
method(s) and save it

16. Select data to batch Process

Highlight Sample Sets, Injections, or
Channels and select process
Standards before Sample & Controls

17. Select the Processing Method/Method Set

(Calibrate and Quantitate) & OK.
Use Clear Calibration to create a new
calibration curve instead of adding points to
an existing curve

23

18. Review the processed results

Highlight the Results Tab, select the desired samples and click the review icon

19. Select the Calibration Curve icon to view Calibration information

24

Order of Calibration Processing

Run Samples**
Calibrate & Report
uses most current
Cal ID will change

Batch Process uses Cal

ID at beginning of
processing
will not change

Review**
Calibrate & Report
uses most current
Cal ID will change

**If you calibrate in Review and save, the data processing in Run
Samples will be affected if using the same processing method

General Rules for Develop Peak

Integration Parameters

Take 2 chromatograms in to Review

Lowest concentration standard or sample for testing

High concentration standard of unknown

Preferable to include a low concentration sample

Will have extraneous peaks needed to be rejected

Peak Integration General Rules

25

Top 10 Calibration Problems

10) Processing different type channels for standards/sample (254 vs 280)

(only works with interchannel processing procedure (MS option enabled
covered in 3D Processing section)
9) Not using clear calibration (points are added to the existing calibration
curve, and not a new curve) incorrect calibration values
8) Not enough data points for calibration curve
(example: Quadratic curve with only 2 calibration points)
7) Point for unknown outside the calibration curve
6) Peak Match ie 2nd Peak selected when no 1st Peak in component table

Top 10 Calibration Problems

5) Internal Standard Peak not found no calibration curve for any components referencing
the Internal Standard
4) Peak falls outside the processing methods components retention time window (use
Show Components)
3) Using the same processing method in Review as in Run Samples during processing
2) Highlighting unknowns before standards when processing (standards must be selected
before unknowns unless using Label and Label Reference)
1) Component names entered in the Amounts button are miss-spelled in the component
table for the processing method
(M32 4.0 with standards will alleviate this problem)

26

The Secrets to Peak Detection

4 ways of Peak Detection

Millennium 3.0 Integration and
Peak Detection basics
Millennium 3.2 Auto peak width &
threshold calculations
Apex Tracking and Inflection
Points
Integration Events

ak Detection 4 Ways
1) You determine Peak Width and Threshold settings**
2) Auto calculation of Peak width and Threshold (3.2)
Enabled in System Policies

3) Peak Apex Tracking Apex

Enabled in Registry, System Policies, Project Properties, and Processing
Processing Method

4) Peak Apex Tracking Inflection Points

**Default M32 Settings

3.2 M32 Settings
* Recommended for regulated environments

27

3.0X Style
Default

3.20 Style
(AutoThreshold)

Basic of Peak Integration Default Way

1) Select the smallest

value in the peak width
box

3) Click the Integrate

icon

2) Box on the
noise & click
on the
Threshold
icon

4) Click on
smallest peak
and click on
Minimum
Height (minimum
area)

28

Basic of Peak Integration

For Integration to occur:

0.00050

Must have a Liftoff (start)

Apex

0.00045

3.974

0.00040
0.00035

Must have an Apex (top)

0.00030
0.00025

AU

0.00020

Must have a Touchdown

(Bottom)

0.00015
0.00010
0.00005

Touchdown

Liftoff

0.00000
-0.00005
-0.00010
-0.00015

3.78

3.80

3.82

3.84

3.86

3.88

3.90

3.92

3.94

3.96

3.98 4.00
Minutes

4.02

4.04

4.06

4.08

4.10

4.12

4.14

4.16

Global Peak Detection Parameters and

Peak Detection Theory

Peak Detection:
Peak Width - Bunching Factor
Threshold slope determination
Peak Integration - Rejection:
Minimum Height (Peak Rejection)
Minimum Area (Peak Rejection)
Understanding the basics of peak detection theory allows you
to set these parameters based on the knowledge of how
those settings will affect peak detection.

29

4.18

Manually Calculating Peak Width Threshold

Step 1 Turn off the Bunching

factor
Select the lowest value listed
in the drop down box
These values will be
determined by the data rate
selected in the Instrument
method

Bunched data points are

used only to detect peaks;
all raw data points are used
for integration.

The Bunching Factor

What is it?

# of Data Points Averaged Together

From the Instrument Method

From the Processing Method

Bunching Factor = Sampling Rate X Peak Width

15

The Magic Number!

Will only be calculated as an Integer

30

The Meaning of Threshold

Threshold & Peak Detection

Threshold value separates
baseline noise from peaks.
Peaks are detected by:
If the average of 2 slopes are
>= threshold value, peak
liftoff is detected.
When the sign of the slope
changes, the peak apex is
detected.
When two slopes are <
threshold value, peak
touchdown is detected.

3.00 Style Peak Width and

Threshold Determination

1.

Threshold and Peak Width

calculated manually
- Manually integrate
smallest peak
- Click on Peak width
- Manually box on largest
baseline noise

2.

Save the processing method

3.

All injections processed will

get the same peak and threshold
values applied

Recommended for regulated

environments threshold and
peak width set once for
complete processing method

31

3.20 Style Peak Width and

Threshold Determination

1.

2.
3.

Threshold and Peak Width

calculated automatically
- Peak width with the
greatest change in slope
- Bunching factor used for
all peaks in channel
Save the processing method
Each injection will have
differing Peak Width and
Threshold values

Not Recommended for regulated

environments threshold and peak
width change for each channel in
processing method

Processing Method - Integration Events

2 Ways to Select Processing Method
Select View Processing Method layout or the
to access integration events

There are 18 different

integration events that
can be applied to
specified time intervals
in your chromatogram

32

icon

Viewing Integration Events

To View the Integration Event Markers- click the
Select Options Show Events

Event Marker Lines

may be moved

Most Common Integration Events

Inhibit Integration
Valley to valley
Allow negative peaks
Exponential Skim
Force Baseline by peak

33

icon or

Integration Inhibit

Enter a start and stop time for Integration Inhibit. Peaks during this time
section will not be integrated or quantitated.
Note: If you want to inhibit after a time, just enter the Time and not
the stop.

Valley to Valley

Valley to Valley Enabled

No Valley to Valley

34

Negative Peaks Integrates

Negative Dips

Before

After

Tangential Skim

Enter a start and stop time for Tangential skim. The Value is the ratio of the parent peak
height to the rider peak height(s) at the valley. The default value for this is 4.
Note: If you want to skim the front peak, use a negative value.

35

Use Options - Fill From Result

Integrated peaks will be filled down in the

component table, by Peak 1, Peak 2, etc. : enter in
component names

Component Names Must be spelled the same as was entered in Run Samples

Global Processing Method

Parameters

Average By: How to calculated points on

the calibration curve if multiple injections
of the same relative concentrations are
used

36

Global Processing Method

Parameters

RT Window (%): Retention time window for each peak as a percentage of

the components retention time. Default: 5%.
CCalRef1: A reference peak for a custom calculation.
Include Internal Standard Amounts in % Amount Calculation:
Specifies if the Internal Standard Amounts are to be included when
calculating %Amount.
Sample Value Type: Specifies if the values entered for calibration in the
Component Editor are concentrations or amounts.

Global Processing Method

Parameters

Update RT: Whether retention time will be

updated in the calibration curve.

37

Retention Time Window

The time window that a peak is still identified as that component.
Retention Time Window can be set 3 ways:
1. Global in % of
RT (default is
5%)
2. Adjust
Component
start/end times to
change RT
Window

3. Manually enter
in RT window
changes

Peak Match

Identification of peaks when multiple peaks are within the same

Component retention Time Window

38

External Standard Calculation

External Standard

RF(X ) =
i

Conc. (X i )std

Response (X i )std

Unknown Concentration

(X ) = RF(
i

Xi )

x Response (X i )

X value (Axis)

Amount ( Actual Amount in a vial)

Concentration (Injection Volume * Amount in the Vial)

39

Y Axis value - Response

Peak Area
Peak Height
Any Peak Related Calculation (custom field)

Fit Type

Select the calibration curve Fit Type - regulated Industries

recommend only Linear or Linear through Zero
Fit Type
# required # Recomm
Linear
2
3
Linear through 0
1
2
Response Factor
1
1
Inverse Linear
2
3
Log-Log Linear
2
3
Point To Point
2
2
Cubic spline
4
6
Quadratic
3
5
Quadratic Thru 0
2
4
Cubic
4
5
Cubic Thru 0
3
4
Fourth
5
6
Fourth Thru 0
4
5
Fifth
6
7
Fifth Thru 0
5
6

40

Weighting Factor
Weighting places more emphasis on the calibration curve points that
have the (smallest deviation - weight).
None

No Weighting

X- X^2, log x , ln X : fit to the points at the high end of the curve (X value).
1/x and1/x^2:

fit to the points at the low end of the curve (X value

1/y and 1/y^2:

fit to the points at the low end of the curve (Y value).

Internal Standards

Internal Standard

41

Internal Standard
Stock Standards

Stock

Internal
Standard

Working Standards

Increasing Solute Concentration

Constant Internal Standard Concentration

Internal Standards

Internal Standard
RFX =
i

Response (I.S.) std

Response (X i ) std

x Conc.(X i ) std

Unknown
(X ) = RF
i

42

Xi

Response (X i )
Response (I.S. )

Retention Time Reference

RT Reference: Adjust the components retention time for the calibration curve based upon the
selected RT Reference component retention time (changes each sample)
The adjusted retention time becomes the time for the component in the chromatogram (the retention
times documented in the processing method are unchanged).
Use this for shifting chromatography
A RT Reference peak also automates two additional calculations - RT Ratio and RRT

Default Peak

Uses the calibration curve of the listed component to calculate

the amount of unknowns that are detected between the Start
and End time listed.

43

Curve Reference

Use designated components calibration curve to

quantitate (calculate amounts) for all other known
components

Relative Resolution Reference

Relative Resolution Reference only appears when System Suitability

option is enabled.
Specifies the Reference peak used to calculate Relative Resolution
equation for System Suitability testing to measure resolution between
named peaks in the Components table and the specified reference peak.

Used for calculation Relative Resolution as part of

system suitability

44

Named Groups

1.
2.
3.
4.

Enter in a Name for the

Group peak
Highlight the Peaks and
drag them to the named
group tree
Select the retention ID
Select how the amounts are
calculated: Sum or User
Entered (User Entered =
Run samples)
The Group peak will be
displayed in the Component
Table as a group
component

Timed Groups

Multiple Components can be grouped according to specific

times as a single component. Millennium32 sums the areas
and heights of the peaks within the specific time period.
Option: Exclude known peaks for example, impurity profiles

45

System Suitability
1.

Enabled Option

2.

Must enter Void

Volume time

Baseline Noise Baseline and Start must be > 30 seconds each side

System Suitability Limits

Set Target and when to calculate limits - limits will be flagged
in the Peaks Table

46

System Suitability Limits

Set Target and when to calculate limits - limits will be flagged
in the Peaks Table

Flagged Peak result

outside of
Retention Time
System Suitability
Limit

Applications of Detector Noise

Signal to Peak to Peak Noise

Example: Uses the detector noise section and custom fields

to calculate ZQ detector noise specification
Height/Average Peak to Peak Noise

47

48